Natural Food Antimicrobial Systems Edited by
A.S. Naidu Director, Center for Antimicrobial Research Department of Food, Nutrition & Consumer Sciences California State Polytechnic University Pomona, California
CRC Press Boca Raton London New York Washington, D.C.
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Library of Congress Cataloging-in-Publication Data Naidu, A. S. Natural food antimicrobial systems / A. S. Naidu. p. cm. Includes bibliographical references and index. ISBN 0-8493-2047-X (alk. paper) 1. Food—Microbiology. 2. Natural products. 3. Anti-infective agents. 4. Antibiosis. I. Title. QR115 N.33 2000 664′.001′579—dc21 00-036053 CIP
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Contents Contributors Preface Chapter 1
Overview A.S. Naidu
SECTION-I
LACTO-ANTIMICROBIALS
Chapter 2
Lactoferrin A.S. Naidu
Chapter 3
Lactoperoxidase A.S. Naidu
Chapter 4
Lactoglobulins E.F. Bostwick, J. Steijns, and S. Braun
Chapter 5
Lactolipids M.F. Lampe and C.E. Isaacs
SECTION-II
OVO-ANTIMICROBIALS
Chapter 6
Lysozyme J.N. Losso, S. Nakai, and E.A. Charter
Chapter 7
Ovotransferrin H.R. Ibrahim
Chapter 8
Ovoglobulin IgY J.S. Sim, H.H. Sunwoo, and E.N. Lee
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Chapter 9
Avidin Y. Mine
SECTION-III
PHYTO-ANTIMICROBIALS
Chapter 10
Phyto-phenols P.M. Davidson and A.S. Naidu
Chapter 11
Saponins W. A. Oleszek
Chapter 12
Flavonoids A.S. Naidu, W.R. Bidlack, and A.T. Crecelius
Chapter 13
Thiosulfinates B.B. Whitmore and A.S. Naidu
Chapter 14
Catechins L.R. Juneja, T. Okubo, and P. Hung
Chapter 15
Glucosinolates B.B. Whitmore and A.S. Naidu
Chapter 16
Agar A.S. Naidu
SECTION-IV
BACTO-ANTIMICROBIALS
Chapter 17
Probiotics A.S. Naidu and R.A. Clemens
Chapter 18
Nisin L.V. Thomas, M.R. Clarkson, and J. Delves-Broughton
Chapter 19
Pediocin B. Ray and K.W. Miller
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Chapter 20
Reuterin M.G. El-Ziney, J.M. Debevere, and M. Jakobsen
Chapter 21
Sakacins F. Leroy and L. De Vuyst
SECTION-V
ACID-ANTIMICROBIALS
Chapter 22
Lactic acid J-C. Bogaert and A.S. Naidu
Chapter 23
Sorbic acid J.N. Sofos
Chapter 24
Acetic acid D.L. Marshall, L.N. Cotton, and F.A. Bal’a
Chapter 25
Citric acid R.K. Sharma
SECTION-VI
MILIEU-ANTIMICROBIALS
Chapter 26
Sodium chloride S. Ravishankar and V.K. Juneja
Chapter 27
Polyphosphates A. Prakash
Chapter 28
Chloro-cides N. Khanna and A.S. Naidu
Chapter 29
Ozone K. Muthukumarappan, F. Halaweish, and A.S. Naidu
Appendix (Symbols and Abbreviations)
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About the Editor
A.S. ‘Narain’ Naidu is a medical microbiologist with more than 20 years of experience in studying the structure-function relationship of antimicrobial agents. He is considered a leading expert on protective and therapeutic applications of natural antimicrobials. As a public health expert, he has served various agencies, including the World Health Organization, the Hungarian Ministry of Health, the Directorate of Medical and Health Services of the Government of India, and the Royal Swedish Academy of Sciences. Dr. Naidu is currently the Director of the Center for Antimicrobial Research, California State Polytechnic University, Pomona. Dr. Naidu received his Ph.D. in Microbiology from the Faculty of Medicine, Osmania University, India, in 1985. His research on staphylococcal enterotoxicosis, toxic shock syndrome and milk lactoferrin in Sweden during the mid-1980s has brought him international recognition. He has published over 50 peer-reviewed scientific papers and about 30 book chapters in this area. In 1997, he moved from the University of North Carolina at Chapel Hill to Cal Poly Pomona, to create a new university research center. Dr. Naidu is principal investigator for a number of scientific projects in the areas of food safety, public health, medicine and dentistry. He also supervises a multi-disciplinary team of scientists and research students.
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Contributors Bal’a, F.A.
Department of Food Science and Technology, Mississippi State University, P.O. Box 9805, Mississippi State, Mississippi 39762, USA.
Bidlack, W.R.
College of Agriculture, California State Polytechnic University, 3801 West Temple Avenue, Pomona, California 91768, USA.
Bogaert, J-C.
Research and Development, n.v. Glactic s.a., 7760 Escanaffles, Belgium.
Bostwick, E.F.
Research and Development, GalaGen Inc., P.O. Box 64314, Saint Paul, Minnesota 55164, USA.
Braun, S.
Research and Development, DMV International Nutritionals, 1712 Deltown Plaza, Fraser, New York 13753, USA.
Charter, E.A.
Research and Development, Canadian Inovatech Inc., 31212 Peardonville Rd., Abbotsford, British Columbia V2T 6K8, Canada.
Clarkson, M.R.
Research and Development, Aplin and Barrett Ltd., 15 North Street, Beaminster, Dorset DT8 3DZ, UK.
Clemens, R.A.
Department of Food Science and Nutrition, California State Polytechnic University, San Luis Obispo, California 93407, USA.
Cotton, L.N.
Department of Food Science and Technology, Mississippi State University, P.O. Box 9805, Mississippi State, Mississippi 39762, USA.
Crecelius, A.T.
Department of Food, Nutrition and Consumer Sciences, California State Polytechnic University, 3801 West Temple Avenue, Pomona, California 91768, USA. Department of Food Science and Technology, University of Tennessee, P.O. Box 1071, Knoxville, Tennessee 37901, USA.
Davidson, P.M. Debevere, J.M.
Department of Food Technology and Nutrition, Faculty of Agricultural and Applied Biological Sciences, Ghent University, Coupure 653, B-9000 Ghent, Belgium.
Delves-Broughton, J.
Research and Development, Aplin and Barrett Ltd., 15 North Street, Beaminster, Dorset DT8 3DZ, UK.
De Vuyst, L.
Research Group of Industrial Microbiology, IMDO, Department of Applied Biological Sciences, Vrije Universiteit Brussels (VUB), Belgium.
El-Ziney, M.G.
Department of Dairy Technology, Faculty of Agriculture, El-Satby, Alexandria University, 5-Aflatone St., Alexandria, Egypt.
Halaweish, F.
Department of Chemistry and Biochemistry, South Dakota State University, Brookings, South Dakota 57007, USA.
Hung, P.
Research and Development, Nutritional Foods Division, Taiyo Kagaku Co., Ltd., Yokkaichi, MIE 510-0825 Japan.
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Ibrahim, H.R.
Department of Biochemical Science and Technology, Kagoshima University, Kagoshima 890, Japan.
Isaacs, C.E.
Department of Developmental Biochemistry, New York State Institute for Basic Research, 1050 Forest Hill Road, Staten Island, New York 10314, USA. Department of Dairy and Food Science, The Royal Veterinary and Agricultural University, Rolighedsvaj 30, DK-1958 Frederiksberg C, Copenhagen, Denmark.
Jakobsen, M.
Juneja, L.R.
Research and Development, Nutritional Foods Division, Taiyo Kagaku Co., Ltd., Yokkaichi, MIE 510-0825 Japan.
Juneja, V.K.
Microbial Food Safety Research Unit, USDA-ARS, Eastern Regional Research Center, 600 E. Mermaid Lane, Wyndmoor, Pennsylvania 19038, USA.
Khanna, N.
Research and Development, Bio-cide International, Inc., P.O. Box 722170, Norman, Oklahoma 73070, USA. Department of Medicine, University of Washington, Box 356523, Seattle, Washington 98195, USA.
Lampe, M.F. Lee, E.N.
Department of Agricultural, Food and Nutritional Science, University of Alberta, Edmonton, Alberta T6G 2P5, Canada.
Leroy, F.
Research Group of Industrial Microbiology, IMDO, Department of Applied Biological Sciences, Vrije Universiteit Brussels (VUB), Belgium.
Losso, J.N.
Department of Food Science, Louisiana State University, Baton Rouge, Louisiana 70803, USA.
Marshall, D.L.
Department of Food Science and Technology, Mississippi State University, P.O. Box 9805, Mississippi State, Mississippi 39762, USA.
Miller, K. W.
Department of Molecular Biology, University of Wyoming, P.O. Box 3354, Laramie, Wyoming 82071, USA.
Mine, Y.
Department of Food Science, Ontario Agricultural College, University of Guelph, Guelph, Ontario, Canada N1G 2W1.
Muthukumarappan, K.
Department of Agricultural and Biosystems Engineering, South Dakota State University, Brookings, South Dakota 57007, USA.
Naidu, A.S.
Center for Antimicrobial Research, California State Polytechnic University, 3801 West Temple Avenue, Pomona, California 91768, USA.
Nakai, S.
Food, Nutrition and Health Program, University of British Columbia, 6650 NW Marine Drive, Vancouver, British Columbia CV6T 1Z4, Canada.
Okubo, T.
Research and Development, Nutritional Foods Division, Taiyo Kagaku Co., Ltd., Yokkaichi, MIE 510-0825 Japan.
Oleszek, W.
Department of Biochemistry and Crop Quality, Institute of Soil Science and Plant Cultivation, 24-100 Pulawy, Poland.
Prakash, A.
Department of Food Sciences and Nutrition, Chapman University, 333 North Glassell Street, Orange, California 92866, USA.
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Ravishankar, S.
National Center for Food Safety and Technology, Illinois Institute of Technology, Moffett Campus, 6502 S. Archer, Summit-Argo, Illinois 60501, USA.
Ray, B.
Department of Animal Science, University of Wyoming, P.O. Box 3354, Laramie, Wyoming 82071, USA.
Sharma, R.K.
Department of Food Science, Michigan State University, East Lansing, Michigan 48823, USA.
Sim, J. S.
Department of Agricultural, Food and Nutritional Science, University of Alberta, Edmonton, Alberta T6G 2P5, Canada.
Sofos, J.
Department of Animal Sciences, Colorado State University, Fort Collins, Colorado 80523, USA.
Steijns, J.
Research and Development, DMV International, NCB-laan 80, 5460 BA Veghel, The Netherlands
Sunwoo, H.H.
Department of Agricultural, Food and Nutritional Science, University of Alberta, Edmonton, Alberta T6G 2P5, Canada.
Thomas, L.V.
Research and Development, Aplin and Barrett Ltd., 15 North Street, Beaminster, Dorset DT8 3DZ, UK.
Whitmore, B.B.
Department of Foods, Nutrition and Consumer Sciences, California State Polytechnic University, 3801 West Temple Avenue, Pomona, California 91768, USA.
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Preface
Food preservation is undoubtedly one of the most significant breakthroughs in human civilization. The technology has been explored for centuries, integrating culinary art with ingredient availability, social necessity, religion and ethnicity. The multifunctionality of natural preservatives, such as herbs, oils and spices, that led to designing a variety of health foods in ancient Asia, Europe and the Mediterranean was well recognized. The evolution of antimicrobial technology, from fermentation to pasteurization, started in wine and cheese factories and extended to revolutionize medicine. Despite our traditional knowledge of natural antimicrobial agents in milk, eggs, plants, probiotics, salts and acids, the structure-function relationship of these bioactive compounds has been unraveled only in the past few decades. We now understand the molecular mechanisms of the ability of a charged cleft in the C-lobe of a milk lactoferrin to bind iron and cause microbial stasis; or the muraminidase activity of a hen egg lysozyme triggering a cidal effect on the cell wall of a Gram-positive bacteria; or the capacity of a galactose-rich polysaccharide in common food-grade agar to detach microorganisms from meat surfaces; or the microbial interference phenomenon and competitive exclusion of pathogens by probiotic bacteria and their bacteriocins; or the pathways of potent oxidative events to break nucleic acid strands and trigger disinfection of viral pathogens by chloro-cides. There is a wealth of knowledge continuously being added to the ocean-depth of common sense we inherited from our ancestors on these fascinating natural food antimicrobials. Emergence of the neo-breed of food-borne pathogens, concerns about the use of synthetic antimicrobials, possibly resulting in the development of microbial resistance, and the global consumer’s awareness of the nutraceutical benefits of natural foods have catapulted the interests of food scientists and food technologists into the ancient art of food preservation. This volume, Natural Food Antimicrobial Systems, is an effort to consolidate the current developments in this area of food science. Although many individuals have extended their help or suggestions in the preparation of this book, several deserve special mention. I am very grateful to my colleague Dr. Wayne Bidlack, Dean, College of Agriculture, California State Polytechnic University, Pomona, for his genuine interest and generous support of my academic endeavors at this institution. I am indebted to Dr. Fergus Clydesdale, Editor, Critical Reviews in Food Science and Nutrition, for recommending this project to CRC Press. Thanks to Lourdes Franco, Associate Editor, Life Science, CRC Press LLC, Boca Raton, Florida, for her professionalism and unstinting support in bringing this book to publication. My appreciation to Gail Renard and associates at CRC Press for expediting the final stages of printing.
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This reference volume is the result of a scientific vision ascending from the click of a mouse to a floppy disk from an illustrious team of scientific experts around the world, both from academia and industry—my sincere appreciation for their relentless effort in contributing the chapters! This project required an in-depth literature search at every level. I would like to commend Erik Ennerberg, Reference Librarian, CalPoly University, Pomona, for providing documentation backup. I also appreciate Thomas Kennedy for drawing the chemical structures. I sincerely thank Brian Dowdle for the desktop design and publishing work. A final note of acknowledgment to my Naidu family: Smita, Tezus, Sreus and Aishwarya for proof reading, cross-referencing and designing the cover. I hope that this volume will contribute to the research and development of the natural food antimicrobial systems and lead to potential applications in nutrition and health.
A.S. Naidu JANUARY 1, 2000
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A.S. Naidu
Overview
1
The effort to process and store food for later use is undoubtedly a quantum leap in the evolution of mankind. It is impossible to establish the exact origins of the development of food processing technology. Anthropological investigations have continuously documented the existence of cooking with fire or some type of food processing dating back to primitive ages. Our interaction with nature and observations of the environment have led to identification of various types of edible foods; antidotes or remedies that cure and protect; as well as an array of flavorants and colorants to please the palate. The integration of such traditional knowledge has turned culinary art into science. The discovery of microorganisms, the so-called ‘animalcules’, in the late 18th century placed food science under the microscope. The power of a microbe such as a milkborne Coxiella burnetti to transmit human disease or the ability of a lactobacillus to ferment milk became evident. Pasteurization became the first-ever science-based antimicrobial food safety measure in dairy processing. The microbiology of food-borne infections and intoxications, as well as food spoilage, has redefined our traditional approaches to food protection. The nutraceutical benefits and the healing power of certain bioactive food ingredients that had been noticed for centuries came under close scientific scrutiny. A multifaceted approach from food science, microbiology, pharmacology and medicine has established ‘Food Antimicrobial Science and Technology’ as an emerging discipline.
FOOD ANTIMICROBIAL TECHNOLOGY Demands and concerns of the global consumer play a critical role in dictating the momentum of research and development in food protection. The demand for minimally processed foods and sustained functionality of naturally occurring bioactive ingredients is steadily rising. This appeal is based on growing concerns about the use of synthetic preservatives with limited documentation on safety and tolerance; the suspected link between the overuse of antibiotics and the development of multi-drug resistance in microbes; and the increased media dissemination of knowledge on diet and health. Furthermore, recent emergence of food-borne pathogens such as the enterohemorrhagic
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Escherichia coli O157:H7, multi-drug resistant Salmonella typhimurium DT104, Listeria monocytogenes, and Enterococcus faecium has made food safety a high priority with the federal, state and local health and regulatory authorities. This is reflected in the President’s National Food Safety Initiative enforced in 1997. Protection of food from spoilers and pathogens can be achieved by various methods including aseptic handling to prevent or minimize microbial entry, removal by physical methods through washing, centrifugation or filtration, destroying with heat, gas or irradiation, and inhibiting growth by refrigeration, freezing, dry packaging, or adding chemical preservatives. Each method is useful as an individual factor in microbial control or is part of a hurdle in a multi-factor food preservation system. This reference volume shall focus on various aspects of ‘Natural Food Antimicrobial Systems’ including molecular aspects of their mechanism of action, influence of factors on structure-function relationships, spectrum of antimicrobial activity, safety and tolerance issues, and more importantly the mass production and feasible application as food ingredients.
NATURAL FOOD ANTIMICROBIAL SYSTEMS Numerous antimicrobial agents exist in animals and plants where they evolved as host defense mechanisms. Naturally occurring antimicrobials are abundant in environment. These compounds may exhibit antimicrobial activity in the foods as natural ingredients or may be used as additives to other foods. The discussion in this reference volume has been limited to six different classes of natural systems. I. LACTO-ANTIMICROBIALS Milk is the first complete functional food devised by nature for the protection and development of a newborn mammal. The prophylactic and therapeutic benefits of milk and its bioactive components have been recognized for centuries. The antimicrobial and nutraceutical potential of many components in milk has been unraveled in recent years. The dairy industry has started isolation of these substances from a variety of sources including cheese whey, hyperimmunized colostrum from cows, and a spectrum of multifunctional applications is being developed in the food and health industry. Lactoferrin (LF) is a metal-binding glycoprotein present in milk and various exocrine secretions that bathe the mucosal surfaces. This natural antimicrobial agent is a multifunctional bioactive molecule with a critical role in many important physiological pathways. LF could elicit a variety of inhibitory effects against microorganisms comprising stasis, cidal, adhesion-blockade, cationic, synergistic and opsonic mechanisms. Broad-spectrum activity against different bacteria, viruses, fungi and parasites, in combination with anti-inflammatory and immunomodulatory properties makes LF a potent innate host defense mechanism. The current commercial production of bovine milk LF is approximately 100 metric tons worldwide and this figure is continuously increasing. This protein is finding its applications as an active ingredient in infant formulae, and health foods in South-East Asian countries, in particular. LF is also in use as a therapeutic and prophylactic agent to control intestinal illnesses and mucosal infections. A number of effi-
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cacy studies and clinical trials are ongoing in various laboratories with over 100 patents filed on this molecule in the past 10 years. Undoubtedly, LF is emerging as one of the leading natural microbial blocking agents in food safety and preservation. Lactoperoxidase (LP) is an oxidoreductase secreted into milk which plays an important role in protecting the lactating mammary gland and the intestinal tracts of the newborn infants against pathogenic microorganisms. LP catalyzes the oxidation of thiocyanate and iodide ions to generate highly reactive oxidizing agents. These products have a broad spectrum of antimicrobial effects against bacteria, fungi and viruses. Microorganisms show great variability in their response to peroxidase systems. The enzymatic properties of LP have found usage in a variety of applications. Its antimicrobial activity has been used to preserve raw milk in warm climates, through the addition of hydrogen peroxide and thiocyanate. Lactoglobulins are potential natural food antimicrobials with a wide spectrum of microbial pathogens and ability to neutralize microbial virulence factors such as toxins. Since colostrum/milk-derived antibodies are polyclonal, they present a multi-faceted approach to pathogen control that transcends the microbial ability to develop resistance mechanisms. Lactoglobulins such as bovine immunoglobulin concentrates have many advantages over synthetic antibiotics: low cost, polyclonal nature in microbial inactivation, activity most likely limited to the intestinal lumen, and less burden on the microbial gut ecology. From a commercial point of view, their entry into the market is rather fast due to less stringent regulatory issues. Lactoglobulin use in dietary supplements or special food products is being considered. Lactolipids are not only nutrients but also antimicrobial agents that are part of an innate defense system functioning at mucosal surfaces. Lipid-dependent antimicrobial activity in milk is due to medium-chain saturated and long-chain unsaturated fatty acids and their respective monoglycerides. The antimicrobial activity of fatty acids and monoglycerides is additive so that dietary-induced alterations in the fatty acid distribution in milk do not reduce lipid-dependent antimicrobial activity. Fatty acids and monoglycerides can rapidly destabilize the membranes of pathogens. The antimicrobial activity of milk lipids can be duplicated using monoglyceride ethers, which very effectively inactivate enveloped viruses, bacteria and protozoa. Monoglyceride ethers are more stable than the ester linkages found in milk lipids since they are not degraded by bacterial or mammalian lipases. Lactolipids and related GRAS (Generally Recognized As Safe) antimicrobial lipids could also be added to infant formulas to reduce the risk of bacterial growth during transport. II. OVO-ANTIMICROBIALS In contrast to the immune system of animals, which produce antimicrobial polypeptides when needed, the egg efficiently resists microorganisms over a long period in the absence of such innate and systemic host defense. Apparently, the main function of ovo-antimicrobials is to keep microorganisms away from the yolk, the nutrient reservoir of egg. The wide diversity in the nature of microorganisms implies that ovo-antimicrobials possess multiple functions. Of many different types of proteins found in the egg albumen, most of them appear to possess antimicrobial properties or certain physiological function to interfere with the growth and spread of the invading microorganisms. © 2000 by CRC Press, LLC
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Lysozyme is a nutraceutical and a value-added product from hen egg white. Singly or in combination with other natural antimicrobial compounds, it has desirable antimicrobial properties for use in minimally processed foods. Lysozyme demonstrates cidal effects on Gram-positive bacteria, however, heat denatured lysozyme has antimicrobial activity against Gram-negative bacteria. Several patents claim the effectiveness of lysozyme, alone or in combination with other synergists, as a food preservative for fruits and vegetables, meat, beverages, and for non-food uses. Food products containing lysozyme, such as cheese, chewing gums, candies, and mouthwashes are on the market. Potential applications in the produce, meat, wine and animal feed industries are increasingly being demonstrated. Ovotransferrin is the major iron-binding protein of egg, which is an equivalent to LF in milk. It acts as a bactericidal agent and its bacterial killing activity can be decoupled from its iron-sequestration properties, in addition to its known bacteriostatic effect (nutritional immunity). Of special interest is that the chemical cleavage at the Asp-X sequence of ovotransferrin produces a strong bactericidal hydrolysate to both Gram-positive and Gram-negative bacteria, heralding a fascinating opportunity for the potential use of the crude hydrolysate in food applications or infant formulas. Ovoglobulin IgY. It has been long recognized that the hen, like its mammalian counterparts, provides young chicks with antibodies as protection against pathogens. This system facilitates the transfer of specific antibodies from serum to egg yolk, and provides a supply of antibodies (IgY class) to the developing embryo and the hatched chicken. The protection against pathogens that the relatively immuno-incompetent newly hatched chick has, is through transmission of antibodies from the mother via the egg. Egg yolk, therefore can be loaded with large amounts of IgY against pathogens which can immobilize the existing or invading pathogens during embryo development or in day-old chicks. Thus, the immunization of laying hens to various pathogens results in production of different antigen-specific IgY in eggs. Egg yolk contains 8-20 mg of IgY per ml or 136 - 340 mg per yolk, suggesting that more than 30 g of IgY can be obtained from one immunized hen in a year. The IgY technology opens new potential market applications in medicine, public health, veterinary medicine and food safety. A broader use of IgY technology could be as a biological or diagnostic tool, nutraceutical or functional food development, oral-supplementation for prophylaxis, and as pathogen-specific antimicrobial agents for infectious disease control. Avidin is a basic tetrameric glycoprotein of egg white. The protein binds up to four molecules of biotin with exceptionally high affinity. This high affinity of avidinbiotin binding has been exploited thoroughly for the development of various molecular tools. Avidin has also been viewed as antibiotic protein in egg albumen inhibiting bacterial growth such as a remedial protein, or as a lytic enzyme. Avidin could inhibit the growth of biotin-requiring yeast and bacteria. The antimicrobial activity also may arise from the ability of avidin to bind various Gram-negative and Gram-positive bacteria. The specific avidin may act as a host defense with antimicrobial and enzyme inhibitor properties. Detailed molecular information through three dimensional structure and protein engineering of avidin would enable us to better understand the biological role and development of avidin as a natural food antimicrobial agent.
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III. PHYTO-ANTIMICROBIALS Phytochemicals exhibiting various degrees of antimicrobial activity occur in plant stems, leaves, barks, flowers, and fruits. Spices and herbs and their essential oils have varying degrees of biological activity. In many cases, concentrations of the antimicrobial compounds in herbs and spices are too low to be used effectively without adverse effects on the sensory characteristics of a food. However, they may contribute to the overall ‘hurdle’ system present naturally in a food product. The most consistent antimicrobial activity among herbs and spices has been found with components of cloves, cinnamon, mustard seed, oregano, rosemary, sage, thyme, and vanillin. Certain phyto-phenolic agents such as oleoresins from olive oil seem to deliver multifunctional physiological benefits to the consumer, and therefore are highly attractive to the health food industry. Since phyto-phenols have been in the food supply and consumed for centuries, these natural phyto-antimicrobials appear to be safe when compared to new synthetic preservatives. Saponins are compounds that protect plants from biotic stress and also elicit antibacterial, antifungal and antiviral activities. This broad-spectrum of antimicrobial activity can be useful in food protection. The ability of saponins to complex with cholesterol in particular may find potential application to lower the diet-induced hypercholesterolemia. Since structurally divergent saponins present different activities, isolation of large quantities of homogenous bioactive form is still a challenge. Flavonoids are extensively characterized by many laboratories for their broadspectrum antimicrobial activity and the lack of resistance induction in target organisms. Isoflavonoids, as natural products and as potent fungal growth inhibitors, could be useful in controlling plant diseases. Due to this high specific antimicrobial activity a possiblie application for isoflavonoids as alternative to conventional fungicides in the control of storage fungi to prevent loss of grains in developing countries has been suggested. Flavonoids are also of great interest in food technology as they contribute to the sensory and nutritional qualities of fruits and fruit products. The antioxidant activity of flavonoids and phenylpropanoids in various beverages including fruit juices is well recognized. Recently, there has been a resurgence of interest in the role of flavonoids in health and disease following the French paradox suggesting an association between reduction in mortality from coronary heart disease and higher wine consumption. Flavonoids are now emerging as potent nutraceutical bioactive food ingredients with sensory appeal to the global food consumer. Thiosulfinates such as allicin and ajoene are the antimicrobial components of garlic. Garlic and its derivatives are multifunctional as well as flavorful food additives. Garlic has been used in the past and is presently being used as a medicine, curative, preservative and a flavoring agent. Thiosulfinates could elicit both cidal and statis effects. Although garlic and its thiosulfinate derivatives appear to be safe for consumption, assessment and protein determination for the allergen responsible for hypersensitivity reactions needs in-depth evaluation. Certain reports have indicated allergic reactions associated with garlic consumption. If thiosulfinates are to be used as preservatives or as antimicrobial agents, the purification techniques and quality control methods need a great degree of standardization.
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Catechins in green tea (GTC) could prevent plaque formation by inhibiting bacterial growth, glucan synthesis and the adherence of carcinogenic streptococci. In addition, GTC could reduce gum disease by suppressing the growth and adherence of periodontal pathogens to buccal epithelial cells as well as by inhibiting the activity of collagenases. GTC also strongly inhibit the growth of intestinal pathogens but do not affect other useful probiotic bacteria. The antimicrobial studies strongly suggest a potential prophylactic role for GTC in human medicine. GTC intake is safe and has health benefits, in addition, green tea is cheap and readily available in fractionated and extracted derivatives. The huge worldwide consumption and safety of GTC may well do significant good and could be supported as an adjunctive therapy and a health ingredient to a good diet, exercise, and avoidance of high-risk behavior. Glucosinolates are abundant in various cruciferous vegetables including cabbage, Brussels sprouts, broccoli, cauliflower, horseradish, mustard, watercress, turnips, radish, rutabaga and kohlrabi. These bioactive compounds have been used for centuries in common herbal preparations and remedies ranging from rheumatism to treating snake poison. As stimulants, mustard and horseradish were applied to oily or high fatty proteins such as fish and meats. Volatile glucosinolates such as the isothiocyanates elicit a wide range of antibacterial and antifungal effects. Application of gaseous allyl isothiocyanates as a preservative in packaged foods has been suggested at low concentrations. A protective anti-tumor association between intake of cruciferous vegetables and cancer of the colon and rectum has been suggested. Broccoli, cabbage and Brussels sprouts were also shown to be protective against mammary carcinogenesis. However, certain studies with purified glucosinolates indicated toxicity in some animal models. Agar is a basic ingredient in the solid-state cultivation of bacteria over most of this century. The possible adsorption of streptococci to the water-soluble galactose fraction from agar warrants attention in interpreting data on bacterial cell surface charge of hydrophobic properties, bacterial adhesion to eucaryotic cells, and agglutination assays for rapid identification of bacteria. The ability to interact with specific mucosal defense factors such as LF and to bind various bioactive compounds makes GRP an excellent immobilizing agent and an antimicrobial delivery system in various food products. IV. BACTO-ANTIMICROBIALS Food fermentation using microbial starter cultures is one of the oldest known uses of biotechnology. Fermented foods and beverages continue to provide an important part of human diet and constitute 20-40% of food supply worldwide. The most common use of probiotics is as food in the form of fermented milk products. Bacteriocins are naturally produced small peptides with bactericidal activity usually against closely related bacteria. Antimicrobial activity of bacteriocins in foods is affected by its levels, type and number of microorganisms, condition of application, interaction/inactivation by food components, and pH and temperature of product. Probiotic strains of lactic acid bacteria (LAB) are generally enteric flora, believed to play a beneficial role in the ecosystem of the human gastrointestinal tract. Recent developments in the role of probiotics (live) and their probioactive (cellular) substances in the intestinal and extra-intestinal physiology of the host are overwhelming. LAB are capable of preventing the adherence, establishment, replication, and/or patho© 2000 by CRC Press, LLC
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genic action of specific enteric pathogens. Probiotic LAB have been used to treat disturbed intestinal microflora and increased gut permeability which are characteristic of many intestinal disorders such as acute rotaviral diarrhea, food allergy, colon disorders, metabolic changes during pelvic radiotherapy and changes associated with colon cancer development. In recent years, consumers have become aware of probiotic properties of cultured milk and dosage specifications. A concentration of 105 cfu/g or ml of the final product has been suggested as the therapeutic minimum. However, the list of probiotic effects and health claims with the use of LAB is expanding. Nisin, a polypeptide bacteriocin produced by Lactococcus lactis ssp. lactis, exhibits antimicrobial activity against a wide range of Gram-positive bacteria associated with food, and is particularly effective against heat-resistant bacterial spores. It is not active against Gram-negative bacteria, yeasts and molds because of its inability to penetrate these cells and gain access to the cytoplasmic membrane. Toxicological studies have found nisin safe and it is now allowed as a food preservative in over 50 countries worldwide. The major use of nisin is in processed cheese, pasteurized dairy products and canned vegetables. In this type of product heat processing eliminates all spoilage microflora except for the nisin-sensitive Gram-positive spore forming bacteria such as bacilli and clostridia. Nisin is also used effectively in combination with heat in crumpets, liquid egg, and fresh soups. Spoilage by LAB can be controlled by nisin in products such as wine and beer, pasteurized vacuum packaged continental sausages, ricotta cheese and acidic foods such as salad dressings and sauces. As part of a hurdle system of preservation nisin can also be used to prevent the growth of pathogens. Current interest is focused on the combination of nisin with novel non-thermal preservation processes such as ultrahigh pressure and electroporation. Pediocins from several strains of Pediococcus acidilactici and Pediococcus pentosaceus, due to their bactericidal property against many Gram-positive bacteria, are explored for their potential use as food preservatives and antibacterial agents. In general, the bactericidal property of pediocins is relatively resistant to heat, storage conditions, pH, organic solvents and hydrostatic pressure, but is destroyed by proteolytic enzymes and neutralized by some anions. The bactericidal action of pediocin PA-1/AcH against target cells is produced through the ability of the molecules to form pores in the membrane and disrupt the proton motive force. Limited studies have shown that pediocin PA-1/AcH, or the producer strain(s), can be effectively used in food systems to control Listeria monocytogenes. Under appropriate processing conditions it can also be used to control Grampositive and Gram-negative spoilage bacteria in foods. Reuterin has been proven to be an effective broad-spectrum antimicrobial able to play a powerful role to improve food safety and prolong shelf life. Further, Lactobacillus reuteri combined with glycerol represents an example of a protective culture which could be added in combination with starter cultures in the manufacturing of fermented fish, sausage, cheese and pickles. This system could control pathogen and spoilage microorganisms during the fermentation process and storage. The efficacy of reuterin as a biopreservative agent and L. reuteri as a protective culture is currently being explored over a wide range of applications. For example, it would be interesting to apply the L. reuteri-glycerol system in highly enriched glycerol foods such as shrimps and other
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seafoods to extend shelf life. The successful use of reuterin as a decontaminating agent for meat and cows’ teat surfaces also suggests more surface disinfectant applications. Sakacins are bacteriocins produced by several strains of Lactobacillus sakei. They are small, cationic, hydrophobic peptides with an antibacterial mode of action against species of lactobacilli and certain food-borne pathogens such as Listeria monocytogenes. Environmental conditions, particularly the pH, will affect sakacin stability and efficacy. Application possibilities are predominantly in the field of sakacin-producing starter or co-cultures for meat fermentations since addition of purified sakacin is not (yet) accepted in food additives legislation. Continued study of the physical and chemical properties and structure-function relationships of sakacins and similar compounds, as well as their in situ functionality either as food additive or being produced by starter, co- or protective cultures is necessary if their potential for future use in meat preservation is to be exploited. V. ACID-ANTIMICROBIALS Several naturally occurring organic acids are added to or are formed in foods through microbial fermentation. Organic acids are amply found in a variety of fruits including apples, apricots, bananas, cherries, citrus varieties, cranberries, grapes, peaches, etc. Acids inhibit microbial growth by lowering the pH, affecting the proton gradient across biological membrane, acidifying the cytoplasm and interfering with the chemical transport across cell membrane. Acid environment not only limits microbial growth but also enhances destruction of microorganisms synergistically with other antimicrobial systems. Most of the approved organic acid antimicrobials, although found naturally in various products, are synthesized chemically as additives of inclusion in food formulations but have a long history of safe use. Organic acids also have been tested or used as washes, sprays, or dips to decrease the microbial load of meat and poultry carcasses. Lactic acid and its derivatives elicit a broad-spectrum of antimicrobial activity against Gram-positive bacteria including spore-forming bacilli and clostridia, as well as Gram-negative pathogens such as enterohemorrhagic E.coli O157:H7 and salmonella. Lactate compounds also demonstrate antifungal activity against aflatoxin-producing Aspergillus sp. Considering these attributes, lactic acid and lactates are widely used in the food industry for decontamination of meat foods such as beef, poultry and pork during processing and packaging. They are also used in shelf life enhancement of fresh and semiprocessed foods. Consumer acceptance of such processed foods, however, is largely based on visual and organoleptic qualities. Currently, the worldwide utility of lactic acid and its derivatives amounts to 100,000 metric tons per year. Sorbic acid use as a preservative relies on its ability to inhibit the growth of various yeasts, molds, and bacteria. Inhibition of microorganisms by sorbates, however, is variable with microbial types, species, strains, food, and environmental conditions. Some microbial strains are resistant to inhibition by sorbate or even metabolize the compound under certain conditions. In addition to being considered less toxic, sorbic acid is also considered more effective than benzoate or propionate in preserving foods such as cheese, fish and bakery products. Sorbates are considered effective food preservatives when used under sanitary conditions and in products processed following GMP.
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Acetic acid and its GRAS salts have a long history of functional use in foods. The ability to lower pH with acetic acid or vinegar provides pickled foods with unsurpassed keeping quality, flavor, and safety. Aside from this traditional use, acetic acid use as a decontaminating agent of fresh and minimally processed foods remains underexploited. Food processors should find acetic acid a desirable functional ingredient or processing aid because of its wide availability, low cost, consumer acceptance, and clean label requirements. Citric acid is produced by most plants and animals during metabolism. The tartness of citrus fruits is due to the citric acid. Lemon juice contains 4 - 8% and orange has about 1% citric acid. Citric acid is widely used in foods, pharmaceuticals, and cosmetics. Citric acid has gained universal acceptance as GRAS ingredient and the Joint FAO/WHO committee has not set any ADI value that makes it a common chemical commodity. Although not a direct antimicrobial agent, citrate is recognized for enhancing the antimicrobial property of many other substances, either by reducing pH or by chelation of metal ions. Its use in controlling thermophiles, in particular, is well established. Citric acid is also used as an antioxidant to prevent oxidative discoloration in foods such as meats, fruits, and potatoes. Citrates of sodium, potassium and calcium also are recognized as GRAS ingredients with a wide range of food applications. VI. MILIEU-ANTIMICROBIALS Traditional antimicrobials include common salt (sodium chloride), sugar and wood smoke that are abundant in the milieu. Common salt has been used as a flavoring or a preservative in foods since ancient times. Curing of meat with impure salt led to the use of nitrates and nitrites as additives for the curing and the preservation of meat products. Exposure to wood smoke is a traditional practice still used in processing. Wood smoke contributes flavor and incorporates antimicrobial compounds such as phenols, formaldehyde, acetate and creosote, into a product. Oxidative damage has been nature’s way of killing microorganisms in phagosomes and an integrated mechanism for antigen processing in various life forms. Various enzyme systems such as oxidases and halide-based catalysts contribute both additive and synergistic effects to numerous natural antimicrobials in the innate host defense. Thus, chloro-cides and ozone could be considered as natural hurdle mechanisms in the physiological milieu. As potent milieu-antimicrobials, chlorocides and ozone could open a powerful hurdle-approach to food safety if integrated with other natural food antimicrobial systems. Sodium chloride, commonly called table salt or salt, is a vital part of human life. Salt enhances the flavor of foods and plays a preserving as well as functional role in food processing. The antimicrobial activity of salt can be both direct or indirect depending on the amount added and the purpose it serves. Since the amount of sodium chloride that must be added to foods to prevent microbial growth is large and will cause an unacceptable taste, it is usually added in combination with other hurdles. The mechanism of inhibition of microorganisms by sodium chloride is mainly by lowering the water activity of the substrate. Studies have also indicated that sodium chloride could have a role in interfering with substrate utilization in microorganisms. The influence of sodium chloride alone as well as its interactive effects with other factors on various microorganisms has
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been well established. However, excessive sodium intake in humans has been linked to hypertension and the related cardiovascular problems and stroke. Hence there are many consumer concerns and the food industry is trying to minimize the salt content of food products. Polyphosphates and their effects on microorganisms in food products depend on various factors which influence their activity such as the concentration, pH, nature of substrate, heat treatment, type and level of microbial contamination, formulation, and storage temperature. Long chain alkaline polyphosphates are more effective as antimicrobial agents compared to short chain polyphosphates, although sodium acid pyrophosphate, a short chain acidic polyphosphate, and trisodium phosphate are very effective in certain applications. The inhibition by sodium acid pyrophosphate is related to the decrease in pH, although pH reduction by itself does not account for suppression of microbial growth. The presence of polyphosphates also appears to increase the sensitivity of several microorganisms to heat. Since polyphosphates function by chelating metal ions essential for microbial growth, in foods with high levels of cations, polyphosphates are not very effective. Gram-positive bacteria and mold are sensitive to polyphosphates and Gramnegative bacteria are resistant to the action of polyphosphates. Level of contamination and age of the culture can also affect polyphosphate action. Synergistic effects have been reported with combinations of polyphosphates and other preservatives such as nitrites and sorbates. Sodium chloride, in some cases, enhances antimicrobial action, and in other cases, decreases effectiveness. Presence of spices may enhance activity. Certain combinations of polyphosphates and other additives such as salt have an additive effect, while other combinations elicit synergism. Polyphosphates lack the broad spectrum of activity exhibited by primary antimicrobials such as sorbate and benzoate. However, as indirect antimicrobials, polyphosphates can impart considerable protection against microbial growth and spoilage while at the same time providing physical and chemical functionality. Chloro-cides are broad-spectrum antimicrobial compounds and oxidative damage is their fundamental mechanism for biocidal action. The biocidal component of most chloro-cides is hypochlorous acid. Currently, the compounds that produce hypochlorous acid are subject to scrutiny because of risks of forming undesired by-products such as trihalomethanes. With major advancements in chemical technology, chlorine dioxide (CD) has emerged as a safe and effective class of chloro-cide. The use of CD as a disinfectant and sanitizer is growing due to its high antimicrobial efficacy and absence of any hazardous by-products. It is extensively used for the treatment of drinking water without adding chlorine taste to the water. CD is also a popular choice of antimicrobial used for the sanitation of produce, poultry, and beef. It is highly effective for the prevention of late blight on potatoes. The recent FDA approval for the use of CD on seafood had provided a useful tool to the food-processing industry for controlling persisting microbial pathogens. Ozone has been used in water purification for decades due to its disinfectant effect on a wide-variety of water-borne pathogens. Numerous studies have indicated that ozone could destroy with extreme efficiency the spores of molds, amoebae, viruses, and bacteria as well as various other pathogenic and saprophytic organisms. Such broad-spec-
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trum and successful use of ozone has created a renewed interest in its utilization as a general germicidal agent. Ozone shows much promise in the food and agriculture industry, however, more research and development is required before its multipurpose usage. Recent GRAS status has encouraged food processors to use ozone for sanitation. Limited data are available on the effect of different concentrations of ozone in reducing bacterial contamination of various food materials and the changes in physical and biochemical characteristics of these foods.
EFFICACY AND APPLICATION Of the many natural antimicrobial systems only a few have been tested or applied to foods. The effectiveness of these antimicrobials depends on a number of factors associated with the target microorganism, the food product, as well as the storage and handling environment. Microbial spectrum. Antimicrobial systems have evolved in nature as specific mechanisms of host defense. Most of these systems are designed to be effective in native existence, and their broad-spectrum of activity is dependent on various factors that regulate the structure-function properties of the antimicrobial agent. Thus, conditions to elicit a potent antibacterial activity such as an iron-depriviation stasis of lactoferrin may not be optimal for a competitive blocking of viral adhesion to an enterocyte. The mechanism of activity also defines the spectrum of an antimicrobial agent. Thus, muraminidase activity would limit the cidal activity of hen egg lysozyme against Gram-positive bacteria. Similarly, nisin is a cationic molecule that interacts with membrane phospholipids of Gram-positive bacteria. However, a synergistic activity with EDTA could make these two antimicrobials effective against Gram-negative bacteria. Various microbial factors also affect the antimicrobial outcome. Actively multiplying vegetative cells at exponential growth phase are more susceptible to an antimicrobial than organisms at stationary growth phase or their sporulating forms. Thus, organisms in an active metabolic state provide ready access to their cellular targets to an antimicrobial agent. However, such proliferating organisms also could develop mechanisms to resist an antimicrobial by shielding cellular targets, producing enzymes that hydrolyze the agent, or induce mutations. Processing conditions could induce heat-shock/acid-shock proteins and convert bacterial outer membrane resistant to antimicrobials. Therefore, the efficacy of a natural antimicrobial system is based on the milieu optima to restore its structure-function, processing conditions and composition of the food product intended for protection. The type of microbial load and intended food safety determines the effective dosage. Food composition. Temperature and pH of the food are the most important factors that influence the antimicrobial activity. Temperature affects the fluidity of the biological membranes and facilitates the perturbation mechanism of hydrophobic antimicrobials. Ionic conditions and pH of the milieu could contribute to the charge alternations and affect antimicrobial interactions with the target surface. Antimicrobials such as lactoferrin, ovotransferrin and lysozyme are cationic in nature and are most effective in acidic pH, a milieu condition that facilitates antimicrobial penetration across the microbial cytoplas-
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mic membrane. Organic acid antimicrobials are weak acids and are most effective in their undissociated form. Thus, weak acids are able to penetrate the cell membrane more effectively in the protonated form, therefore, the pKa value of these compounds is important in selecting a particular compound for an application. Thus, the lower the pH of a food product, the greater the proportion of acid in its undissociated form and the greater the antimicrobial activity. Polarity of the antimicrobial molecule is also an important characteristic; thus, side groups such as the alkyl, benzyl moieties could enhance the ionization of phytoantimicrobials such as the flavonoids, saponins, and glucosinolates. Most food antimicrobials are hydrophobic in nature, a physical property that facilitates their interaction with surfaces. Presence of certain lipids or proteins in certain foods may bind to an antimicrobial via non-specific hydrophobic interaction and inactivate them by immobilization. The antimicrobial activity of thiosulfinates from garlic and certain bacteriocins is compromised in high-lipid milieu. Oxidative antimicrobial activity of chloro-cides and ozone decreases in organic environment, protein-rich in particular. Delivery system. An antimicrobial is added to a food processing line by various techniques such as a direct incorporation to the product formulation; spray or immersion of the product in an antimicrobial solution; dusting a dry powder of the antimicrobial over the product; application to the packing material that comes in contact with the food; or applying a multi-compound formulation with carriers such as vegetable oil, ethanol or propylene glycol. The mode of application for a specific product depends on type of food product; properties of the antimicrobial; type of processing; and expected efficacy. The delivery system selected should be compatible with the bio-functionality of the antimicrobial agent. Cost factor. The extraction of bioactive antimicrobials from natural sources can be complex and expensive. Selection of natural source, isolation and commercial application is challenging due to the complexity of food, the variety of factors influencing preservation, and the complex chemical and sensory properties of natural antimicrobials. Nondenaturing extraction procedures, efficient large-scale isolation methods, and techniques to retain bio-functional properties are being optimized for most natural antimicrobials described in this volume.
REGULATORY ISSUES Toxicological problems associated with the use of certain synthetic food antimicrobials has generated interest in the food industry for use of naturally occurring compounds. Commonly used antimicrobials, such as organic acids that are produced in large quantities through chemical synthesis, are also found naturally in many food products and are GRAS according to regulatory authorities. Many natural food ingredients are time tested with proven benefits as food additives; however, this does not warrant a safety claim for specific components isolated from these materials. Isolation of bioactive components from a natural source poses new parameters of safety evaluation for the following reasons: 1) the isolation process might enrich an undesirable allergen, mutagen or toxin from a natural source; 2) an otherwise non-toxic component might be activated during isolation; 3) the extraction/purification methods possi-
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bly may denature a bioactive component and create a new artifact with toxic manifestations; 4) residual solvents or elution chemicals might react and/or contaminate the final product and compromise the structure-functional properties; 5) the level of acceptable daily intake of an isolated biological compound could be higher than its consumption via natural source; 6) the purified natural antimicrobial when incorporated in a formulation might react with other ingredients to form toxic species. Therefore, all naturally occurring antimicrobials should demonstrate safety either by animal testing or by continuous consumption by consumers as a food over a long period. In addition to lacking toxicity, they must be non-allergenic and be metabolized and excreted and should not lead to residue build-up. Food antimicrobials should not react either to make important nutrients unavailable or destroy these nutrients. Their potential impact on the sensory characteristics of a food must be considered. Compounds that negatively affect flavor and odor or contribute inappropriate flavor and odor would be unacceptable.
PERSPECTIVE In an attempt to satisfy the rapidly changing consumption patterns of the global market, the food processing industry is continuously developing various new and modified products. Such product development requires cutting-edge technology to ensure organoleptic distinction as well as other qualities such as wholesomeness, sanitary grade, shelf-life, and safety. Development of convenience foods, functional diets, nutraceutical health supplements also has necessitated the use of additives and antimicrobials. Many of the natural food antimicrobial systems also demonstrate a multifunctional physiological advantage and are emerging as value-added ingredients in various food products. Milk lactoferrin is now being explored as an antioxidant, an iron-delivery system and an immuno-modulating agent in various sports drinks and infant formulations. Globulin-rich ingredients such as whey-protein concentrates and hen egg proteins seem to reduce gastric ulcers in controlled clinical trials. Phyto-antimicrobials including thiosulfinate concentrates from garlic and oleuropeins from olives are suggested to lower cholesterol; catechins from green tea were shown to prevent gum disease; and flavonoids from cranberry were reported to lower the incidence of urinary tract infections. Lactic acid bacteria are believed to induce a probiotic effect and thereby improve gut physiology that might even contribute to the prevention of intestinal carcinogenesis. Many such natural food antimicrobial systems are currently used in a variety of over-the-counter remedies. Antimicrobial-flavorants including oleoresins of spices, vanillin, diacetyl and organic acids; antimicrobial-colorants such as turmeric, kola, anthocyanins, diterpenes, and stilbenes could serve as dual-function food additive systems. The application potential of natural food antimicrobial systems is enormous. The scientific basis for incorporation into various foods and the technical knowledge for the biofunctional maxima of natural food antimicrobial systems are currently being explored worldwide.
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LITERATURE RECOMMENDED 1.
Board, R.G., and Dillon, V. 1994. Natural Antimicrobial Systems in Food Preservation. Wallingford, UK: CAB International. 2. Davidson, P.M., and Branen, A.L. 1993. Antimicrobials in Foods. 2nd Edition. New York: Marcel Dekker. 3. De Vuyst, L., and Vandamme, E.J. 1994. Bacteriocins of Lactic Acid Bacteria. New York: Chapman and Hall. 4. Doyle, M.P., Beuchat, L.R., and Montville, T.J. 1997. Food Microbiology – Fundamentals and Frontiers. Washington, D.C: ASM Press. 5. Gould, G.W. 1989. Mechanisms of Action of Food Preservation Procedures. London: Elsevier Applied Science. 6. Gould, G.W. 1995. New Methods of Food Preservation. Glasgow, UK: Blackie Academic and Professional. 7. Hoover, D.G., and Steenson, L.R. 1993. Bacteriocins of Lactic Acid Bacteria. San Diego, California: Academic Press. 8. Jay, J.M. 1998. Modern Food Microbiology. 5th Edition. Gaithersburg, Maryland: Aspen Publishers. 9. Naidu, A.S., Bidlack, W.R., and Clemens, R.A. 1999. Probiotic spectra of lactic acid bacteria. Crit. Rev. Food. Sci. Nutr. 39:13-126. 10. Ray, B., and Daeschel, M.A. 1992. Food Biopreservatives of Microbial Origin. Boca Raton, Florida: CRC Press. 11. Russel, N.J., and Gould, G.W. 1991. Food Preservatives. London: Blackie and Son Ltd. 12. Sofos, J.N., Beuchat, L.R., Davidson, P.M., and Johnson, E.A. 1998. Naturally Occurring Antimicrobials in Food. Task Force Report No.132. Ames, Iowa: Council for Agricultural Science and Technology.
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Section-I LACTO-ANTIMICROBIALS
Lactoferrin Lactoperoxidase Lactoglobulins Lactolipids
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I. INTRODUCTION Lactoferrin (LF) is an iron-binding glycoprotein present in milk and many exocrine secretions that bathe the mucosal surface. Though the term ‘LF’ implies an ironbinding component in milk, this molecule co-ordinately binds to various metal ions and occurs in divergent biological milieu including saliva, tears, seminal fluids, mucins, and the secondary granules of neutrophils. LF has a multifunctional role in a variety of physiological pathways and is considered a major component of the preimmune innate defense in mammals. The ability of LF to bind two Fe+3 ions with high affinity in cooperation with two HCO3- ions is an essential characteristic that contributes to its major structure-functional properties including antimicrobial activities. Iron is a transition metal belonging to group VII elements in the periodic table; it occurs at an approximate level of 2-g in the body of normal human adults and is essential for all living organisms. The ability of iron to alternate between its two valency states is its most important biological property, and is used in many metabolic pathways including the bioenergetic coupling of inorganic phosphate to adenosine phosphate (ADP) to form adenosine triphosphate (ATP). Nevertheless, this property can be hazardous for the cell, as it can lead to generation of reactive oxygen species. Under controlled conditions, however, iron is used beneficially, e.g., by the phagocytes in intra-lysosomal killing of microorganisms. Various iron-binding proteins have evolved in the animal physiological system to sequester iron from the milieu. Ovotransferrin (conalbumin) from the egg white was the first iron-binding protein to be purified (Osborne & Campbell, 1900). In 1939, Sörensen and Sörensen identified a red iron-binding protein in bovine milk. Later, Schafer (1951) also reported a similar protein in human milk termed ‘siderophilin’. Schade and Caroline (1946) isolated an iron-binding protein from human serum (serotransferrin) which was later named ‘transferrin (TF)’. In 1960, Groves from the United Kingdom, Johansson from Sweden, Montreuil and co-workers from France, and Gruttner and co-workers from Germany independently isolated the red milk protein ‘lactosiderophilin’ from milk.
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Natural Food Antimicrobial Systems
During the 1960s several investigators isolated and characterized this protein from various exocrine secretions and tissues of humans and animals (Gordon et al., 1963; Blanc et al., 1963; Masson et al., 1965a; 1965b; 1965c; 1966; 1969; Masson & Heremans, 1968). Based on structural and chemical homology with serum TF, Blanc and Isliker (1961a; 1961b) proposed the name ‘lactoferrin’ for this protein. Though LF is not exclusively found in milk, this name is now widely recognized in the scientific community, although the term ‘lactotransferrin’ can be found in earlier publications. LF was isolated as a major component in the specific granules of the polymorphonuclear leukocytes (PMNLs) with an important role in the amplification of inflammatory responses (Masson et al., 1969; Baggiolini et al., 1970; Oseas et al., 1982; Boxer et al., 1982a; 1982b; 1982c; Lash et al., 1983; Ambruso et al., 1984; Brittigan et al., 1989). LF has also been reported to be a component of the sperm-coating antigen (Ashorn et al., 1986) and was found to have cross-reactivity and sequence homology with the major histocompatibility antigen (Aguas et al., 1990). Extensive work by Masson and his Belgian group has established a clear role for LF in cellular immunity and has led to the identification of specific LF-receptors on macrophages, intermediation of endotoxic shock and hyposideremia (Van Snick et al., 1974; Van Snick & Masson, 1976). Pioneering efforts by Spik, Montreuil and their French group unraveled the biological chemistry of LF (Mazurier et al., 1981; Spik et al., 1982; Metz-Boutigue et al., 1984). Lönnerdal has opened the nutritional role for LF in the absorption of metal ions in the intestinal tract (Davidson & Lönnerdal, 1986; Davidson et al., 1990; 1994). In 1978, Broxmeyer and coworkers reported a regulatory function for LF in myelopoiesis (Broxmeyer et al., 1978; 1984). In 1961, Oram and Reiter reported the ability of milk LF to inhibit the growth (stasis effect) of Bacillus sp. and found that nutritional deprivation of the bacteria from iron accounted for the antimicrobial activity. The antimicrobial spectrum of LF was further elucidated by Brock’s group (Brock et al., 1978; 1983; Brines & Brock, 1983). In 1977, Arnold and co-workers reported cidal activity for LF against a variety of microorganisms at acidic pH and noted that it is not inhibited by salts in the media (Arnold et al., 1977; 1980; 1981). Despite wide citation in literature, the cidal effect of native LF appears to be artifactual in nature, caused by reactants other than LF in the milieu (Lassiter, 1990). The research group at the Morinaga Milk Company in Japan found that acid/pepsin hydrolysis of bLF could generate cationic antimicrobial peptides ‘lactoferricins (LFcins)’ (Tomita et al., 1989; 1991; 1994; Bellamy et al., 1992; 1993). This broad-spectrum cationic microbial killing seems to be non-specific and readily inhibited by salts in the milieu at physiological concentrations. Erroneously, LFcins are widely described in the literature as bactericidal domains, implying they are peptides responsible for the antimicrobial effect reported by Arnold’s group. Interaction of LF with specific targets on the microbial surface causes an array of outcomes either to the advantage of the host (microbial blocking effects) or the microorganism (iron-acquisition and pathogenesis). Naidu and co-workers have identified, isolated and characterized LF-binding microbial targets in a variety of Gram-positive and Gram-negative bacteria (Naidu et al., 1990; 1991a; 1991b; 1992; 1993). Specific high-affinity interaction of LF with pore-forming outer membrane proteins (OMPS) of Escherichia coli, in particular, has unraveled a molecular mechanism for antimicrobial activity which seems to be well conserved in
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Gram-negative enterics (Kishore et al., 1991; Tigyi et al., 1992; Erdei et al., 1993; Naidu & Arnold, 1994). The LF-mediated outer membrane damage in Gram-negative bacteria reported by Ellison et al. (1988) has explained certain antimicrobial effects such as antibiotic potentiation, release of lipopolysaccharides (LPS) and alterations in microbial OM permeation. The critical role of iron in the pathogenesis of many microbial infections has been widely advocated (see reviews: Weinberg et al., 1975; Bullen, 1981). Thus, the mobilization of iron from physiological milieu from LF, TF and ferritin by pathogens appeared to be an important virulence trait. Rogers and Synge (1978) reported a siderophore-mediated mobilization of iron from LF by E.coli. Another type of iron-acquisition mechanism involving specific receptors was reported by Alderete’s group as well as Sparling and co-workers, as a virulence factor in various intracellular pathogens, in particular, among the etiological agents of sexually transmitted diseases (Mickelsen et al., 1982; Peterson & Alderete, 1984; Biswas & Sparling, 1995). Later, Schryvers’ group identified and characterized a number of specific receptors for LF on various mucosal pathogens (Schryvers & Morris, 1988; Schryvers, 1989). This chapter is mainly confined to the antimicrobial spectrum of milk LF and its possible role in food safety and preservation. The multifunctionality of LF is also described to emphasize its nutraceutical benefits as a value-added food ingredient.
II. OCCURRENCE A. Normal levels In the human body, LF occurs in two major reservoirs, a circulatory pool stored in the polymorphonuclear lymphocytes (PMNL) and a stationary pool on the mucosal surfaces. In PMNL, LF is associated with the secondary (specific) granules at a concentration of about 15 µg/106 cells (Baggiolini et al., 1970; Bennett & Kokocinski, 1978) and is released isochromously with other lysosomal proteins into the plasma during phagocytosis (Bennett & Skosey, 1977; Leffell & Spitznagel, 1975). LF content in plasma is low or undetectable during agranulocytosis (Bennett & Kokocinski, 1978) and neutropenia (Hansen et al., 1975; Olofson et al., 1977), thus suggesting that PMNL are the sole source of intravascular LF production. The concentration of LF in human plasma is about 0.2 to 1.5 µg/ml (Rumke et al., 1971); the values are comparatively lower in women than in men (Bennett & Mohla, 1976). The plasma LF levels are also low in children due to reduced PMNL secretion (Gahr et al., 1987). LF is rapidly eliminated from the plasma with a mean fractional catabolic rate of 5.7/day, by liver and spleen; however, apo-LF is removed at a slower rate of 1.22/day (Bennett & Kokocinski, 1979). Hirai and co-workers (1990) measured LF concentration in human milk and colostrum from 1 to 60 days after parturition (125 samples) by rocket immuno-electrophoretic assay using anti-hLF antiserum. The LF concentrations in colostrum (1-3 days of puerperium, n = 35), the transitional milk (4-7 days, n = 60), and mature milk (20-60 days, n = 30) were about 6.7, 3.7, and 2.6 g/L, respectively. Both the LF and total protein (TP) concentrations showed inverse correlation with the days after parturition. The LF/TP ratio in the mature milk (16.1%) was significantly less than that in the colostrum (20.4 %) and the transitional milk (21.4%). Furthermore, iron concentration in human milk was also measured by the internal standard technique of the spiked method on atomic absorp-
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tion, and the LF iron-saturation was calculated. Neither Fe nor iron-saturation % showed a significant difference among these three stages of lactation. The means (n = 125) of Fe and iron-saturation % were about 0.61 µg/ml and 11.8%, respectively. However, significant correlation was observed between LF and Fe or between LF/TP and both Fe and TP in the mature milk. These results suggest that the mechanism stimulating the synthesis and secretion of LF is different from those of other proteins and LF can play variable roles in iron nutrition of infants during different stages of lactation. An immunoperoxidase staining technique was used for detecting LF, TF and ferritin in routine histological paraffin sections of human tissue. LF was found in lactating breast tissue, bronchial glands, PMNLs, and gastric and duodenal epithelial cells (Mason & Taylor, 1978). The expression of LF was studied in human gastric tissues displaying normal, benign hyperplastic or malignant histology (Luqmani et al., 1991). A single 2.5kb mRNA was detected in only 14% (2/14) of normal resections. This was similar to the finding that 85% of tumors were also negative, with 4/27 positive. In contrast, samples with superficial or atrophic gastritis had a high frequency of expression, with 5/7 and 9/14 positive, respectively. The higher incidence of LF mRNA in antral samples was a reflection of the greater proportion of these compared with body resections of patients with gastritis. No expression was seen in any of 5 gastric carcinoma cell lines. High levels were observed in the cardia, in contrast to complete absence in the oesophagus. Immunocytochemistry showed localization of LF in cells of both antral and body glands. Chief cells, but not adjacent parietal cells, were strongly stained. In tissues exhibiting superficial or atrophic gastritis a greater degree and intensity of staining was observed as compared with samples with normal histology LF accounts for about 11.5% of the total secretary proteins of the bronchial glands (Harbitz et al., 1984). In these glands, LF is uniformly distributed in large amounts in the serous cells and is restricted only to the basal part of cytoplasm in the mucus cells (Masson et al., 1966). LF is released into the nasal secretions by serous cells of submucosal glands under the influence of the parasympathetic nervous system (Raphael et al., 1989). In human tears, LF is synthesized in the lacrimal glands (Janssen & van Bijsterveld, 1982; 1983) at a concentration of 1 to 3 mg/ml that accounts for ~25% of the total tear protein (Kijlstra et al., 1983). In the male reproductive tract, LF is found in the prostate, seminal vesicles, and seminal plasma (0.2 to 1.0 mg/ml), but not in testis (Rumke, 1974; Wichmann et al., 1989). As the sperm-coating antigen, LF may suppress lymphocyte response against sperm (Ashorn et al., 1986). It may also partially account for the antimicrobial and immune-suppressive activity of the seminal fluid in the female reproductive tract before and during fertilization (Broer et al., 1977). In the female reproductive tract, LF has been detected in the cervical mucus and endometrium of the secretory uterus (Tourville et al., 1970) B. Clinical levels Acute phase host responses such as an inflammation or toxic shock result in the depletion of iron from plasma (Klasing, 1984). The interleukin 1 (IL-1) seems to mediate multiple aspects of acute phase response and also induce exocytosis of PMNLs to release intracellular granule contents, including LF (Klempner et al., 1978; Dinarello, 1984). Eventually, the plasma LF levels increase in various pathological conditions and its estimation may serve as a prognostic marker. Thus, the elevated plasma LF level is an early
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indicator of septicemia and endotoxemia (Gutteberg et al., 1988). During meningococcal septicemia, LF level in the serum and cerebrospinal fluid is elevated within 18 h of onset as to the same magnitude of the C-reactive protein (Gutteberg et al., 1984). Similarly, an increase in the plasma and serum LF levels during cystic fibrosis seems to correlate with the intensity of the cystic fibrosis protein (Barthe et al., 1989). The estimation of elevated LF concentration with cholecytokinnin secretin (CCK-S) test has been suggested to improve the differential diagnosis of chronic pancreatitis (Dite et al., 1989). LF to lysozyme ratio in the crevicular fluid may be helpful in the diagnosis of localized juvenile periodontitis (Friedman et al., 1983). In the pathogenesis of rheumatoid arthritis, iron has an important role in the degradation of intact cartilage matrices, due to its capacity to generate free radicals that activate latent collagenases (Blake et al., 1981; 1984; Bukhhardt & Schwingel, 1986). Elevated levels of LF in the synovial fluids and synovial membranes due to inflammatory tissue damage is a characteristic of this disease (Ahmadzadeh et al., 1989). This high LF concentration has been suggested in the regulation of subsequent inflammatory processes critical for articular damage. Neoplastic cells have an increased iron-requirement for the initiation and maintenance of DNA synthesis and for cell multiplication (Gatter et al., 1983; Barresi & Tuccari, 1987). In different types of malignancies, iron uptake may be mediated by specific receptors for LF or TF. Immunohistochemical studies have demonstrated LF in adenocarcinomas of the parotid gland (Caselitz et al., 1981), well differentiated prostatic carcinomas, breast carcinomas (Charpin et al., 1985), thyroid carcinomas of follicular origin (Tuccari & Barresi, 1985; Barresi & Tuccari, 1987), renal cell carcinomas (Loughlin et al, 1987), intestinal-type carcinomas, and incomplete intestinal metaplasia (Tuccari et al., 1989).
III. ISOLATION AND PURIFICATION LF from bovine milk was first isolated by Groves (1960). Various procedures for isolation of LF from mammalian milk have been reported. The most commonly used methods include chromatographic separation on CM-Sephadex, Cibacron Blue F3G-ASepharose, Heparin agarose and single stranded DNA agarose (FIGURE 1). A. Size-exclusion chromatography on CM-Sephadex columns Gel filtration is one of the earlier techniques used for isolation of LF from various biological secretions (Butler, 1973). Tsuji and co-workers (1989) described a method to isolate LF from bovine colostrum. Colostrum obtained within 24 h after parturition was centrifuged at 3000 rpm for 10 min and 1 liter of the skimmed colostrum was dialyzed against distilled water in the presence of 0.01% sodium azide for 3 days at 4°C with several changes of distilled water. The dialyzed skimmed colostrum was loaded on a CMSephadex C-50 (Pharmacia) column (2 x 20 cm) equilibrated with 0.05 M potassium phosphate buffer, pH 8.0 (buffer-A). LF was eluted with a linear gradient of NaCl (0.1 to 0.7 M) in buffer-A after unbound proteins and weakly bound proteins were washed out sequentially with 100 ml of buffer-A and 100 ml of buffer-A containing 0.05 M NaCl. The combined fraction containing LF was dialyzed against buffer-A at 4°C overnight and reloaded onto a column of CM-Sephadex C-50 (1 x 5 cm). LF was eluted with a linear gradient of NaCl (0.2 to 0.5 M) in buffer-A, and at this step, 192 mg of nearly homogenous LF was obtained. © 2000 by CRC Press LLC
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FIGURE 1. LF isolation methods - elution profiles on different chromatography columns [redrawn from Tsuji et al., 1989; Furmanski et al., 1989; Rejman et al., 1989; Hutchens et al., 1989].
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B. Affinity-chromatography on Cibachron Blue-Sepharose columns Various laboratories have adapted this method to isolate LF from human milk (Arnold et al., 1977; Bezwoda & Mansoor, 1986; Furmanski et al., 1989; Shimazaki & Nishio, 1991). Briefly, 5 ml of pooled human milk is skimmed and decaseinated by centrifugation (10,000 g, 40 min), acidification (to pH 4.7 with HCl), heating (40°C, 30 min) and recentrifugation (10,000 g, 40 min). The milk whey is dialyzed overnight against 500 ml veronal buffer. The whey was diluted to 25 ml with veronal buffer. The sample was applied to Cibachron Blue Sepharose CL-6B (Pharmacia) column (1 x 10 cm). The column is washed with 25-ml veronal buffer and eluted with a 30-ml linear gradient of 0.51 M NaCl in veronal buffer. A single protein peak corresponding to LF elutes at about 0.75 M NaCl. The radioisotope labeled 59Fe-saturated LF demonstrated an elution pattern similar to apo-LF during this separation method (Furmanski et al., 1989). C. Affinity-chromatography on heparin-cross linked columns Heparin-agarose affinity chromatography has been used to isolate LF from human milk whey in a single chromatographic step (Blackberg & Hernell, 1980). AlMashikhi and Nakai (1987) have used heparin-sepharose affinity chromatography to isolate LF from cheddar cheese whey. In this procedure, whey is dialyzed against 0.05M NaCl in 0.005 M sodium barbital-HCl buffer, pH 7.4. Whey solution is applied to a heparin-agarose column equilibrated with the above dialysis buffer. Protein is eluted at a flow rate of 48 ml/h using a continuous gradient of 0.05M to 1.0 M NaCl constituted in the dialysis buffer. Fractions are collected and absorbance is read at 280 nm. Rejman et al. (1989) used this method to isolate bLF from mammary secretions collected during the nonlactating period. About 1600 absorbance units (280 nm) of whey protein were efficiently separated by the heparin-agarose column (packed with 2.0 x 16.5 cm of Affi-Gel heparin agarose from Bio-Rad) into four absorbance peaks. LF was identified in the fourth peak (eluting at a conductivity of 30 mS). Both iron-saturated and apo-forms of LF demonstrated similar elution profiles in this technique. IgG1 and secretory component are the trace contaminants with bovine milk whey fractionation. In contrast, serum albumin was identified as the contaminant with human milk whey separation on the heparin column. D. Affinity-chromatography on DNA-agarose columns Hutchens and co-workers (1989) reported that immobilized DNA is effective for a rapid and complete purification of apo-LF and holo-LF from colostrum in a single step. Urea was utilized as a mobile phase modifier to eliminate the interaction of other proteins such as serum albumin both with LF and with the immobilized DNA. Briefly, in this method, single-stranded DNA-agarose is packed into a 1.0 x 1.5 cm column to a bed volume of 5 to 10 ml. The column is washed with water, then equilibrated with 20 mM Hepes buffer, pH 8.0, with or without 6 M urea, at a flow rate of 30 ml/h. The separation procedure is performed at room temperature. Solid urea ( up to 6 M) is added before the sample (5 to 10 ml) is applied to the DNA affinity column. The column is washed with equilibration buffer and prior to gradient elution, urea (if present) is removed with several column volumes of 20 mM Hepes buffer, pH 8.0 (HB). LF is eluted with a linear gradient of NaCl (0 to 1.0 M) in 20 mM HB. Fractions of 1 ml each are collected and the absorbance
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was measured at 280 nm. The radioisotope labeled 59Fe-saturated LF demonstrated an elution pattern similar to apo-LF during this separation method. Finally, after each purification procedure the DNA-agarose column was washed extensively, first with 2 M NaCl in HB, followed by 8 M guanidine-HCl in HB and finally with water. Iron saturation and desaturation: Various methods of iron saturation (holoform) and desaturation (apo-form) of LF have been described. Briefly, apo-LF is prepared by dialysis against an acetic acid/sodium acetate buffer (pH 4.0), followed by exhaustive dialysis against deionized distilled water (Mazurier & Spik, 1980). Holo-LF is prepared by adding a large excess of citric acid (pH 2.5; 60 mol citric acid:1 mol iron). After incubation for 10 min, the pH is raised to 7.0 with 0.1 M NaOH. Excess sodium bicarbonate is added (2 mol bicarbonate:1 mol iron). Unbound iron is removed by gel filtration (Azari & Baugh, 1967). Masson and Heremans (1968) described a method to prepare apo-LF. A concentration of 1% LF solution was deprived of iron by dialysis against 20 volumes of 0.1 M citric acid. After 36 h the citrate was eliminated by dialysis against 20 volumes of deionized water for 2-h at 4°C. The required amount of solid disodium phosphate was added to the dialysis flask. Stirring was discontinued and the flask was kept at 4°C. The pH of the suspension increased slowly as the crystals of disodium phosphate dissolved into the solution. This precaution is needed to prevent precipitation of the protein. Stirring is resumed as soon as the pH in the upper layer of buffer has reached a value of 5.0. The final pH is 7.6. After such treatment, the solution of LF turns completely colorless. Fe(III) removal from LF by an Fe(III)-chelating resin with immobilized 3hydroxy-2-methyl-4(1H)-pyridinone ligands at physiological pH in the presence of citrate has been described (Feng et al., 1995). The resin had a marked effect on the extent of iron removal. By using the Fe(III)-chelating resin, removal of iron from LF was nearly complete in < 24 h. Apo-LF with 4% iron saturation could be prepared conveniently from 100% or from 18% iron-saturated LF under mild conditions without affecting the ironbinding capacity of the protein.
IV. MOLECULAR PROPERTIES A. Physico-chemistry The physico-chemical characteristics of hLF and bLF are listed in TABLE 1. Like the transferrins of blood serum and egg white, LF is a single polypeptide chain with a molecular weight in the range 75 to 80-kDa. Dry weight determinations together with measurement of iron-binding capacities, showed combining weights per iron atom bound of 39,000 for bLF, and 40,000 for hLF (Aisen & Leibman, 1972). Accordingly, these correspond to molecular weights of 78,000 and 80,000 daltons, respectively, for protein molecules with two specific binding sites. The isoelectric point (pI value) of bLF is reported at about 8.0 by free boundary electrophoretic methods (Groves, 1960; Szuchet-Drechin & Johanson, 1965); pI of 8.8 by Rotafors method (Shimazaki et al., 1993) and a pI of 8.2-8.9 by chromatofocusing (Shimazaki et al., 1993). On the otherhand, a wide range of pI values, from 5.5 to 10.0 have been reported for hLF by isoelectric focusing techniques [5.8 to 6.5 by Bezwoda & Mansoor, 1989; 6.9 by Malmquist & Johanson, 1971; 8.7 by Moguilevsky et al., 1985; 8.8
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TABLE 1. Lactoferrin – Physico-chemical properties Property Molecular mass Sedimentation co-efficient SDS-PAGE Iron titration Isoelectric point Chromato focusing Isoelectric focusing Absorption spectra Apo-form at 280 nm Holo-form at 470 nm Glycosylation Protease sensitivity IgA-complexes Iron-binding Equilibrium dialysis (K1 x 10-4) Thermal denaturation Apo-LF denaturation (Tmax: °C) Apo-LF enthalpy (∆Hcal: J/g) Holo-LF denaturation (Tmax: °C) Holo-LF enthalpy (∆Hcal: J/g)
Human LF
Bovine LF
Reference
75,100 76,800 + 1,600 80,000
77,200 + 1,300 76,000 + 2,400 78,500
6.8 – 8.0 5.8 – 6.5
8.2 – 8.9 9.5 – 10.0
Castellino et al., 1970 Querinjean et al., 1971 Aisen & Leibman, 1972 Bezwoda & Mansoor, 1989 Yoshida & Xiuyun, 1991 Shimazaki et al., 1993 Aisen & Leibman, 1972
10.9 0.510 Relatively high Relatively low Present
12.7 0.400 Low High Absent
26.0
3.73
Metz-Boutigue et al., 1984 Brines & Brock, 1983 Watanabe et al., 1984 Aisen & Leibman, 1972 Paulsson et al., 1993
71 + .3 & 90 + .3 12 + .4 & 2 + .5 65 + .3 & 93 + .3 2 + 1 & 37 + 1
to 8.9 by Birgens & Kristensen, 1990; and 8-10 by Kinkade et al., 1976]. By the Rotafors method hLF was focused at a pI of 8.7 and by chromatofocusing the hLF was eluted at pH 6.8-8.0 (Shimazaki et al., 1993). Heat-induced enthalpy changes in different forms of bLF in water were examined by differential scanning calorimetry (Paulsson et al., 1993). Two thermal transitions with varying enthalpies were observed, depending on the iron-binding status of the protein. Iron-saturated holo-LF was more resistant to heat induced changes than the apoform. Investigations of metal-substituted hLF by fluorescence, resonance Raman, and electron paramagnetic resonance (EPR) spectroscopy confirm the close similarity between LF and serum TF (Ainscough et al., 1980). As in the case of Fe(III)- and Cu(II)TF, a significant quenching of apo-LF’s intrinsic fluorescence is caused by the interaction of Fe(III), Cu(II), Cr(III), Mn(III), and Co(III) with specific metal binding sites. Laser excitation of these metal-LFs produce resonance Raman spectral features at about 1605, 1505, 1275, and 1175 cm-1. These bands are characteristic of tyrosinate to the metal ions, as has been observed previously for serum TF, and permit the principal absorption band (lmax between 400 and 465 nm) in each of the metal-LFs to be assigned to charge transfer between the metal ion and tyrosinate ligands. Furthermore, as in serum TF the two metal binding sites in LF can be distinguished by EPR spectroscopy, particularly with the Cr(III)-substituted protein. Only one of the two sites in LF allows displacement of Cr(III) by Fe(III). LF is known to differ from serum TF in its enhanced affinity for iron. Accordingly, the kinetic studies show that the rate of uptake of Fe(III) from Fe(III)-citrate is 10 times faster for apo-LF than for apo-TF. Furthermore, the more pronounced conformational change which occurs upon metal binding to LF is corroborated by the production of additional EPR-detectable Cu(II) binding sites in Mn(III)-LF. The lower pH required for iron removal from LF causes some permanent change in the protein as judged
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by altered rates of Fe(III) uptake and altered EPR spectra in the presence of Cu(II). Thus, the common method of producing apo-LF by extensive dialysis against citric acid (pH 2) appears to have an adverse effect on the protein. The anion binding properties of hLF, with Fe(III) or Cu(II) as the associated metal ion, highlight differences between the two sites, and in the anion binding behavior when different metals are bound (Brodie et al., 1994). Carbonate, oxalate and hybrid carbonate-oxalate complexes have been prepared and their characteristic electronic and EPR spectra recorded. Oxalate can displace carbonate from either one or both anion sites of Cu2(CO3)2 LF, depending on the oxalate concentration, but no such displacement occurs for Fe2(CO3)2 LF. Addition of oxalate and the appropriate metal ion to apo-LF under carbonate-free conditions gives dioxalate complexes with both Fe3+ and Cu2+. Both the carbonate and oxalate ions bind in bi-dentate fashion to the metal, except that the carbonate ion in the N-lobe site of dicupric LF is mono-dentate. The hybrid copper LF complex shows that the oxalate ion binds preferentially in the C-lobe site in a bi-dentate mode. Overall these observations lead to a generalized model for synergistic anion binding by TF and allow comparisons to be made with non-synergistic anions such as citrate and succinate. The amino acid composition of LF molecules isolated from the milk of different mammalian species is shown in TABLE 2. Tryptic peptide maps of hLF show some 40 spots, which is a much smaller number than would be predicted from the lysine and arginine content (Querinjean et al., 1971). LF is a glycoprotein containing two glycans attached through N-glycosidic linkages. The two N-acetyl-lactosaminic-type glycans are structurally heterogenous (Spik et al., 1982) and differ from those of other transferrins (Spik et al., 1975; Dorland et al., 1979; Van Halbeck et al., 1981). Analysis of bLF for carbohydrate content reveals 1 residue of terminal sialic acid, 10 to 11 residues of N-acetyl TABLE 2. Lactoferrin - Amino acid composition of protein isolated from different species Amino acid Aspartate Threonine Serine Glutamate Proline Glycine Alanine Cysteine Methionine Valine Isoleucine Leucine Tyrosine Phenylalanine Tryptophan Lysine Histidine Arginine
Human
Bovine
Porcine
Monkey
Murine
Equine
71 31 50 70 35 56 63 32 6 49 16 61 20 31 11 46 9 46
71 39 45 73 31 43 59 28 4 43 17 61 19 25 9 42 10 32
57 28 46 71 30 50 56 X 4 42 18 53 20 26 X 40 8 36
72 31 43 67 34 61 73 23 2 50 15 62 29 30 X 47 9 40
71 40 50 71 33 51 60 28 5 45 17 57 18 25 10 55 10 32
72 32 48 70 33 50 71 38 3 44 14 60 20 25 12 45 10 33
Adapted from Hutchens et al., 1989
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glucosamine, 5 to 6 residues of galactose, and 15 to 16 residues of mannose per molecule (Castellino et al., 1970). In hLF, according to the sequence studies by Metz-Boutigue et al., 1984), asparagine residues 137 and 490 are glycosylated. Prediction of the secondary structure suggested that the two prosthetic sugar groups were linked to asparagine residues located in a β-turn conformation. The non-glycosylated asparagine residue 635 also occurs in a β-turn whereas asparagine residue 389 is located in a region of non-predictable structure. Spik et al. (1982) elucidated the primary structure of glycans from hLF. The polypeptide chain of hLF consists of two glycoslyation sites to which glycans are linked through an N-(β-aspartyl)-N-acetylglucosaminylamine bond and which are structurally heterogenous. After chymotryptic or pronase digestions, glycopeptides with five different glycan structures were isolated. Three of these structures were determined by using methanolysis, methylation analysis, hydrazinolysis/nitrous deamination/ enzymatic cleavage and 1H-NMR spectroscopy at 360 MHz. Glycopeptides-A/B: NeuAc(α-26)Gal(β-1-4)GlcNAc(β-1-2)Man(α-1-3)[NeuAc(α-2-6)Gal(β-1-4)GlcNAc(β-12)Man(α-1-6)]Man(β-1-4)GlcNAc(β-1-4)[Fuc(α-1-6)]GlcNAc(β-1-)Asn;Glyco-peptideC:NeuAc(α-2-6)(Gal(β-1-4)GlcNAc(β-1-2)Man(α-1-3)(Gal(β-1-4)[Fuc(α-1-3)] GlcNAc(β-1-2)Man(α-1-6))Man(β-1-4)GlcNAc(β-1-4)[Fuc(α-1-6)]GlcNAc(β-1-)Asn. Glycopeptide-D:NeuAc(α-2-6)Gal(β-1-4)GlcNAc(β-1-2)Man(α-1-3)[Gal(β-14)GlcNAc (β-1-2)Man(α-1-6)]Man(β-1-4)Glc-NAc(β-1-4)[Fuc(α-1-6)]GlcNAc(β1)Asn. The other two glycopeptides were obtained in very low amounts with more complex structures. It is generally believed that each iron-binding site contains two or three tyrosine residues (Windle et al., 1963) and one or two histidine residues (Krysteva et al., 1975; Mazurier et al., 1981); and concomitantly bound bicarbonate ion (Schlabach & Bates, 1975) may be held electrostatically to an arginyl side group (Rogers et al., 1978). B. Structure LF is a member of the iron-binding protein family collectively known as transferrins (TF). Human LF demonstrates amino acid sequence homology (more pronounced in the C-terminal region) with serum hTF (59%) and hen ovotransferrin (49%). Computer analysis has established an internal homology of the two lobes (residues 1-338, and 339703), each containing a glycosylation site (aspargine residues 137 and 490) located in homologous position (Metz-Boutigue et al., 1984). Each lobe has a capacity to bind one Fe+3 ion with high affinity (Kd =10-20 M-1) in the presence of a carbonate or bicarbonate anion (Harris, 1986). It has been suggested that the iron-binding site contain two or three tyrosine residues (Windle et al., 1963; Teuwissen et al., 1972) and one or two histidine residues (Mazurier et al., 1981); the concomitantly bound bicarbonate anion (Schlabach & Bates, 1975) may be held electrostatically to an arginyl side group (Rogers et al., 1978). Baker and co-workers have extensively studied the three-dimensional structure of LF (FIGURE 2).The hLF molecule at 3.2-Å resolution has two-fold internal homology. The N- and C-terminal halves form two separate globular lobes, connected by a short alpha-helix, and carry one iron-binding site each (Anderson et al., 1987). The two lobes of the molecule have very similar folding; the only major differences being in surface loops. Each lobe is subdivided into two dissimilar α/β domains, one based on a six-stranded mixed β-sheet, the other on a five-stranded mixed β-sheet, with the iron site in the inter-domain cleft. The two iron sites appear identical at the present resolution. Each iron
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FIGURE 2. LF molecule: A schematic diagram. Helices are shown as cylinders, β-strands as arrows, iron atoms , probable anion sites ❍, disulfide bridges , and carbohydrate attachment sites (labeled L for lactoferrin, T for serum transferrin, O for ovotransferrin, and M for melanotransferrin). The N-terminal half (N-lobe) is at top, the C-terminal half (C-lobe) at bottom; their relative orientations, related by a two-fold screw axis are shown in the inset. The two domains in each lobe are labeled 1 and 2. A region where hydrophobic interactions between the two lobes are made is indicated (H). Helices labeled are the connecting helix (A) and the C-terminal helix (B) [from Baker et al. (1987) with permission from the Elsevier Publications].
atom is coordinated to four protein ligands, 2 tyrosine, 1 aspartate, 1 histidine, and the specific CO32-, which appears to bind to iron in a bi-dentate mode. The anion occupies a pocket between the iron and two positively charged groups on the protein, an arginine sidechain and the N terminus of helix 5, and may serve to neutralize this positive charge prior to iron binding. A large internal cavity, beyond the arginine side-chain, may account for the binding of larger anions as substitutes for CO32-. Residues on the other side of the iron site, near the inter-domain crossover strands, could provide secondary anion binding sites, and may explain the greater acid-stability of iron binding by LF, compared with serum TF (Anderson et al., 1989).
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X-ray structure analyses of four different forms of hLF (diferric, dicupric, an oxalate-substituted dicupric, and apo-LF), and of bovine diferric LF, have revealed various ways in which the protein structure adapts to different structural and functional states (Baker et al., 1991). Comparison of diferric and dicupric LFs revealed that different metals, through slight variations in the position, have different stereo-chemistry and anion coordination without any significant change in the protein structure. Substitution of oxalate for carbonate indicated that small side-chain movements in the binding site could accommodate larger anions. The multi-domain nature of LF also allows rigid body movements. The structure of apo-LF demonstrated the importance of large-scale domain movements for metal binding and release and suggested equilibrium between open and closed forms in solution, with the open form being the active binding species. The crystal structure of a site-specific mutant of the N-terminal half-molecule of hLF(N), in which the iron ligand aspartate-60 has been mutated to serine, was studied to determine the effects of the mutation on iron binding and domain closure (Faber et al., 1996). At the mutation site the serine side-chain neither bound to the iron atom nor made any inter-domain contact similar to the substituted aspartate; instead a water molecule filled the iron coordination site and participated in inter-domain hydrogen bonding. The domain closure was also changed, with the mutant with a more closed conformation. Consideration of crystal packing suggested that the altered domain closure is a genuine molecular property but both the iron coordination and inter-domain contacts were consistent with weakened iron binding in the mutant. The role of conserved histidine ligand in iron binding of LF was studied by sitedirected mutagenesis and X-ray crystallographic analysis (Nicholson et al., 1997). His253 in the N-terminal half-molecule of hLF (residues 1-333) was changed to Gly, Ala, Pro, Thr, Leu, Phe, Met, Tyr, Glu, Gln, and Cys by oligonucleotide-directed mutagenesis. The mutant proteins were expressed in baby hamster kidney cells, at high levels, and purified. The study indicated that the His ligand is essential for the stability of the iron binding site. All of the substitutions destabilized iron binding irrespective of whether the replacements were potential iron ligands or not. Iron was lost below pH approximately 6.0 for the Cys, Glu, and Tyr mutants and below pH 7.0 or higher for the others, compared with pH 5.0 for the N-terminal half molecule. The destabilization was attributed to both steric and electronic effects. The decreased stability of the iron binding was attributed solely to the loss of the His ligand as the protein conformation and inter-domain interactions were unchanged.
FIGURE 3. Comparison of N-terminal sequences of LF molecule from different mammalian species.
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The three-dimensional structure of diferric bLF and factors that influence its iron binding were reported (Moore et al., 1997). The final model comprised 5310 protein atoms (residues 5 to 689), 124 carbohydrate atoms (from ten monosaccharide units, in three glycan chains), 2 Fe3+, 2 CO32- and 50 water molecules. The folding of bLF molecule was similar to that of hLF, but bovine species differed in the extent of closure of the two domains of each lobe, and in the relative orientations of the two lobes. Differences in domain closure were attributed to amino acid changes in the interface, and differences in lobe orientations to slightly altered packing of two hydrophobic patches between the lobes. Changed inter-domain interactions were implied to the lesser iron affinity of bLF, compared with hLF, and two lysine residues behind the N-lobe iron site of bLF offer new insights into the ‘dilysine trigger’ mechanism proposed for iron release by TFs. The bLF structure was also notable for several well-defined oligosaccharide units that demonstrate the structural factors that stabilize carbohydrate structure. One glycan chain, attached to Asn-545, appears to contribute to inter-domain interactions and possibly modulate iron release from the C-lobe. C. Heterogeneity Among mammalian LFs, the human protein has been widely characterized. The amino acid and cDNA sequence data indicate that several animal LFs share extensive regions of primary sequence homology. Specifically, N-terminal sequences for porcine LF (Hutchens et al., 1989) indicate homology between LFs from human (Metz-Boutigue et al., 1984), bovine (Wang et al., 1984), equine (Jolles et al., 1984), monkey (Davidson & Lönnerdal, 1986) and murine (Pentecost & Teng, 1987) origins (FIGURE 3). X-ray diffraction studies also have demonstrated certain degrees of structural homology between hLF and bLF molecules (Norris et al., 1986). Peptide mapping also suggested structural homology between porcine and human LFs (Kokriakov et al., 1988). LFs isolated from various sites of the human body demonstrate antigenic similarity. Considering the total amino acid sequence (Metz-Boutigue et al., 1984) and the polydispersity of the glycan structures (Spik et al., 1982), hLF has an estimated molecular mass of 82,400 + 400. However, hLF in a number of human body fluids was found to possess different electrophoretic mobility due to its interaction with acidic macromolecules (Hekman, 1971). Several reports have also suggested polymerization of LF to a variable degree in biological fluids. Different forms of LF seem to appear at distinct stages of certain infections. Tabak et al. (1978) have detected LF polymers in the saliva of a patient with acute parotitis, however, apparent dimers and monomers were recovered when the inflammation gradually subsided. Similarly, bLF trimers appear in milk during acute stages of bovine mastitis, while dimers and eventually monomers emerge as predominant forms during the healing process (Harmon et al., 1976). The LF aggregation phenomenon in calcium containing fluids seems to inactivate certain biological activities of the molecule, such as the feedback control of granulopoiesis (Bennett et al., 1981). Three isoforms of hLF with identical molecular mass, pI, partial proteolytic peptide patterns, and N-terminal amino acid sequence, but with distinct RNAse activity, were reported. The LF-alpha form binds iron; and, the other two, LF-beta and LF-gamma forms, express potent RNAse activity but lack the iron binding capacity (Furmanski et al., 1989). Two apparent forms of LF were also identified in bovine colostrum and the molecular heterogeneity seems due to a varying degree of protein glycosylation (Tsuji et al., 1989).
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V. ANTIMICROBIAL EFFECTS Structural characteristics and spatial orientation of the molecule are critical factors in the functionality of an antimicrobial compound. Occurrence in various milieu strongly emphasizes the significance of the structure-function relationship in the multifunctionality of the LF. As an exocrine secretory protein LF is present in different biological fluids of varying viscosity, pH, and ionic strength and co-exists with continuously changing ratios of other physiological substances. Thus, LF may be expected to perform a different antimicrobial function in the tear or saliva compared to its activity against an enteric bacteria at the intestinal mucosa. Moreover, as an acute-phase reactant LF also exists as a regulatory molecule in the cellular pool such as the neutrophils, and contributes to antigen processing in the phagosomes. Considering the diversity of LF’s role in innate defense, a broad-spectrum of antimicrobial activity is expected. Accordingly, various modes of antimicrobial effects have been reported for LF. A. Stasis effect The iron-chelating capacity of LF in the metal-binding pockets in co-ordination with the bicarbonate anion has been suggested in the nutritional deprivation and a consequent inhibition of microbial growth in the stasis effect. This hypothesis was supported with various laboratory findings, such as exogenous addition of iron into the milieu could reverse the stasis effect or iron-saturated LF is non-inhibitory. During the early 1960s, Reiter’s laboratory suggested the stasis mechanism of antimicrobial action for LF, which was further substantiated by Masson and co-workers. The stasis effect has been verified and validated by various laboratories during the past three decades. There are vast numbers of peer-reviewed publications in the scientific literature and this section will discuss the salient points. Kirkpatrick et al. (1971) reported the fungistatic effect of apo-LF against Candida albicans and suggested a role for LF in the host-defense mechanism in chronic mucocutaneous candidiasis. Reiter et al. (1975) found that two strains of E. coli were inhibited by colostral whey after dialysis or dilution in Kolmer saline and addition of precolostral calf serum or LF. Undiluted dialyzed milk was not inhibitory due to its low LF content but became inhibitory after addition of 1 mg/ml of LF. The lack of inhibition in undiluted whey is due to the high concentration of citrate in colostral whey (and milk) and it is suggested that citrate competes with the iron-binding proteins for iron and makes it available to the bacteria. Addition of bicarbonate, which is required for the binding of iron by TF and LF, could overcome the effect of citrate. Bishop et al. (1976) tested the bacteriostatic effects of apo-bLF against strains of coliform bacteria associated with bovine mastitis. As low as 0.02 mg of apo-bLF per ml resulted in marked inhibition of growth of all coliforms. The stasis effect was lost if saturated LF or iron plus apo-LF was added to the synthetic medium. The inhibition of growth increased as the concentration of apo-LF increased from 0.02 to 0.2 mg/ml for Klebsiella pneumoniae and 2 mg/ml for Aerobacter aerogenes, and E. coli. As the concentration of apo-LF was increased above 0.2 or 2 mg/ml, there was less inhibition of growth except for E. coli. These results are compatible with the hypothesis that coliform bacteria respond to low-iron environments by production of iron-sequestering agents that compete effectively with apo-LF for free iron. Addition of apo-LF plus citrate resulted in
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loss of growth inhibition. The molar ratio (citrate to apo-LF) was found to be more important than the absolute concentration of either component. A ratio of 75 resulted in 50% growth inhibition, whereas ratios of 300 and greater resulted in less than 10% growth inhibition. These results suggest that the ratio of citrate to LF would be important in evaluating LF as a nonspecific protective factor of bovine mammary secretions. An in vitro microassay was developed to evaluate bacteriostatic properties of apo-bLF (Nonnecke & Smith, 1984a). The growth of coliform, staphylococcal, and streptococcal bacterial strains in a defined synthetic medium was inhibited by apo-bLF (0.5 to 30.0 mg/ml). Addition of holo-LF to the synthetic medium did not inhibit growth of test strains. Inhibition by apo-LF was greater for coliform than Gram-positive strains for all concentrations of apo-LF evaluated. No concentration of apo-LF proved bactericidal for either coliform or Gram-positive strains. Inhibition of two coliform strains by apo-LF (10 mg/ml) was abolished by addition of ferric iron to the assay system, indicating an irondependent nature of apo-LF induced inhibition of bacteria. Bicarbonate supplementation of the growth system containing apo-LF (1 mg/ml) increased inhibition of three coliform strains by apo-LF. Addition of increasing concentrations of citrate (2.0 mg/ml) to an assay system containing apo-LF (5 mg/ml) resulted in a concomitant reduction of growth inhibition of three coliform strains. These data confirmed a potential relationship between the molar ratio of citrate to LF of the lacteal secretion and its capacity to inhibit coliform strains associated with mastitis. Mammary secretions were collected during physiologic transitions of the udder and were used in an in vitro microbiological assay to determine bacteriostasis of mastitis pathogens (Breau & Oliver, 1986). As mammary involution progressed, in vitro stasis of Klebsiella pneumoniae, E. coli, and Streptococcus uberis increased. Mammary secretions from concanavalin A (conA)- and phytohemagglutinin (PHA)-treated glands had significantly increased bacteriostasis. Secretions contained significantly increased concentrations of LF and a decreased citrate:LF molar ratio earlier in the dry period than did control mammary secretions. Greatest bacteriostasis was observed in mammary secretions obtained 7 days before parturition. However, differences in secretion composition or bacteriostasis were not found between conA- or PHA-treated and control udder halves during the prepartum period. Bacterial growth inhibition by mammary secretion decreased markedly during early lactation. A highly significant positive correlation was found between bacteriostasis and concentrations of LF, serum albumin, and IgG. A highly significant negative correlation was also reported in the citrate:LF molar ratio during early involution and the peripartum period. The bacteriostasis effect bLF, TF and immunoglobulins against E. coli strain B117, acting alone or in combination, was investigated in vitro (Rainard, 1986a). Both LF and TF elicited a strong bacteriostasis without requirement for antibodies. After a short period of growth, the multiplication of bacteria was almost completely prevented by the iron-binding proteins. A significant but moderate additional stasis was achieved when IgG or IgM was added to TF, while addition of Ig to LF revealed no significant cooperative effect. All of 11 strains of E. coli isolated from bovine mastitis were sensitive to LF in the absence of Ig. It therefore appeared that antibodies were not required for LF to exert a potent bacteriostatic effect on mastitis isolates of E. coli. Rainard (1986b) also examined the bacteriostatic activity of bLF against mastitis pathogens using an in vitro microassay. The most susceptible species was E. coli; all of the 35 isolates tested were susceptible to
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bacteriostasis by apo-LF (0.1 mg/ml), although a few strains showed a lower degree of inhibition. Heterogeneity among strains was more pronounced among 10 isolates of Staphylococcus aureus, four of which were apparently unaffected by apo-LF (1 mg/ml). Under the same conditions, Streptococcus agalactiae (six isolates) and Strep. uberis (five isolates) resisted the bacteriostatic action of apo-LF. The growth of Streptococcus mutans 6715-13 in a rich medium (Todd Hewitt broth) was drastically reduced by addition of apo-LF; this effect was bacteriostatic and reversible by saturation of LF with iron (Visca et al., 1989). Dionysius et al. (1993) examined the in vitro antibacterial effects of various forms of LF on enterotoxigenic strains of E. coli using a microassay for bacterial growth. Native and apo-LF exhibited variable activity against 19 strains, whereas holo-LF had no effect. At a concentration of .2 mg/ml of apo-LF, strains could be distinguished as either sensitive or resistant to inhibition. Zinc-saturated LF was as bacteriostatic as apo-LF when sensitive and resistant strains were tested over the concentration range .04 to 1.0 mg/ml of LF. A bactericidal effect was observed for native, apo-, and Zn-saturated LF against some sensitive strains. The antibacterial activity of apo-LF depended on bacterial inoculum size and was not enhanced by the addition of lysozyme. Addition of holo-LF or cytochrome c diminished the antibacterial effect of apo-LF, whereas addition of BSA had no effect. Resistance to inhibition by LF was not related to the production of bacterial siderophores. Paulsson et al. (1993) tested the effect of pasteurization- and UHT-treatments on the LF interaction with bacteria. The ability of native and iron-saturated LF to bind various bacterial species was unaffected by pasteurization. However, UHT treatment decreased this interaction capacity. Native LF, both unheated and pasteurized, showed similar bacteriostatic properties and moderately inhibited E. coli. However, this inhibitory capacity was lost after UHT treatment. Iron-saturated LF did not inhibit bacterial growth; neither pasteurization nor UHT could change this property. Thus, UHT seems to affect structural as well as certain biological properties (including bacteriostasis) of both native and iron-saturated bLF, and pasteurization seems to be a treatment of choice for products containing this protein. The effect of LF on bacterial growth was tested by measuring conductance changes in the cultivation media by using a Malthus-AT system and was compared with the magnitude of 125I-labeled LF binding in 15 clinical isolates of E. coli (Naidu et al., 1993). The binding property was inversely related to the change in bacterial metabolic rate and was directly related to the degree of bacteriostasis (FIGURE 4). The magnitude of LFbacterium interaction showed no correlation with the MIC of LF. In certain strains, LF at supraoptimal levels reduced the bacteriostatic effect. Thus, the LF concentration in the growth media was critical for the antibacterial effect. The cell envelopes of Salmonella typhimurium 395MS with smooth lipopolysaccharide (LPS) and its five isogenic rough mutants revealed 38-kDa porin proteins as peroxidase-labeled-LF-reactive components in sodium dodecyl suLFate-polyacrylamide gel electrophoresis and Western blot (ligand blot) analysis. However, in the whole cell-binding assay, parent strain 395MS demonstrated a very low interaction with 125I-LF. On the other hand, LF interaction gradually increased in correspondence with the decrease in LPS polysaccharide moiety in the isogenic rough mutants. Conductance measurement studies revealed that the low-level-LFbinding (low-LF-binding) strain 395MS with smooth LPS was relatively insusceptible to LF, while the high-LF-binding mutant Rd was more susceptible to LF (FIGURE 5). These
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FIGURE 4. LF binding to E.coli and its relation to antimicrobial outcome. Correlation between parameters was made by linear regression analysis. The metabolic rate in the presence of LF (1 mg/ml) is expressed as a relative percentage, considering the change in the conductance rate of the control (without LF) as 100%. Bacteriostasis was estimated as the difference between bacteria growth in media with LF and the control. For MIC determinations, bacteria were grown in the presence of 15 different concentrations of LF within a range of 0.01 to 10 mg/ml. The lowest amount of LF that caused complete inhibition of bacterial growth at the time point when the metabolism of the control reached stationary phase was considered as MIC [reproduced from Naidu et al. (1993) with permission from the American Society for Microbiology].
data suggested a correlation between LF binding to porins and the LF-mediated antimicrobial effect. The polysaccharide moiety of LPS shielded porins from the LF interaction and concomitantly decreased the antibacterial effect. Dial et al. (1998) have examined the in vitro and in vivo antimicrobial efficacy of bLF against Helicobacter species. LF was bacteriostatic to H. pylori when cultured at concentrations above or 0.5 mg/ml. Growth of H. pylori was not inhibited by another milk constituent, lysozyme, or by bLFcin, but growth was inhibited by the iron chelator deferoxamine mesylate. LF inhibition of growth could be reversed by addition of excess iron to the medium. LF in retail dairy milk was found to be more stable intra-gastrically than unbuffered, purified LF. Treatment of H. felis-infected mice with LF partially reversed mucosal disease manifestations. The authors concluded that bLF has a significant antimicrobial activity against Helicobacter species in vitro and in vivo. The growth of Bacillus cereus was markedly inhibited by the addition of LF and was recovered by the addition of FeCl3 (Sato et al., 1999). The bacteriostasis was also reversed by the addition of erythrocytes and hemoglobin. B. cereus could use heme or heme-protein complex (hemoglobin-haptoglobin and hematin-albumin complexes) as iron sources in iron deficient conditions. Thus, B. cereus seems to use such heme or hemeprotein complexes to prevent the bacteriostasis of LF in vivo. B. Cidal effect In 1977, Arnold and co-workers reported a bactericidal effect for native LF molecule, which apparently was distinct from the stasis mechanism. These experiments were performed with microbial cells suspended in deionized water or buffer solutions at acid pH and the reported mechanism is controversial. Various laboratories have failed to demonstrate a similar bactericidal effect (Rainard, 1987; Gutteberg et al., 1990). Lassiter (1990), from Arnold’s group, later published a doctoral thesis which indicated that conta-
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FIGURE 5. Growth of S. typhimurium 395MS(S) (S; parent with smooth LPS) and its isogenic mutant Rd (with rough LPS) in SPYE broth. Control ( ), with 1 mg/ml bLF (❍) and 5 mg/ml bLF ( ). [Redrawn from Naidu, et al., 1993].
mination of EDTA during dialysis of LF could account for the cidal effect against E.coli. Furthermore, the cidal effects of LF against oral streptococci seem due to the acid pH of the test system. Degradation products in an LF preparation such as the cationic peptides could elicit membrane damage and kill microorganisms. In an antimicrobial milieu such as in the phagosome, LF could possibly elicit a cidal effect synergistic with oxidative events. However, clear evidence for a direct cidal effect with native (intact) LF molecule in vitro is still lacking. This section has reviewed the cidal effect in a chronological perspective with no endorsement for the mechanisms hypothesized in the literature. LFs seem to elicit cidal effects against a variety of microorganisms including Gram-positive and Gram-negative bacteria, rods and cocci, facultative anaerobes, and aero-tolerant anaerobes. Similar morphological and physiological types are represented among the LF-resistant bacteria (Arnold et al., 1980). S. mutans was more resistant to LF when grown on a sucrose-containing medium than when it was grown on brain heart infusion broth without added sucrose. When an LF-sensitive, avirulent strain of Streptococcus pneumoniae was passed through mice, the resultant virulent culture demonstrated resistance to LF. Since organisms of the same species and even of the same strain such as S. pneumoniae, can differ in susceptibility to LF, it appears that accessibility to the LF target site may account for variations in susceptibility. Influence of several physical conditions and the metabolic state of Streptococcus mutans on LF susceptibility were reported (Arnold et al., 1981). After exposure to LF, a 15-min lag period occurred before the initiation of killing, indicating that a two-step process is involved in LF killing. Cultures harvested during the early exponential phase were sensitive to LF, whereas cultures harvested in the early stationary phase were markedly resistant. The rate of killing was dependent on temperature; there was no loss of viability at 2ºC. Killing occurred at pH 5.0 to 6.0 in water and 20 mM glycine, but not at any pH in 50 mM sodium phosphate or N-2 hydroxyethylpiperazine-N’-2-ethanesulfonic acid (HEPES) buffer. Addition of exogenous ferrous or ferric ions did not reverse or prevent LF killing, nor did 1 mM magnesium chloride.
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Bactericidal effect of LF against Legionella pneumophila was reported (Bortner et al., 1986). Purified apo-hLF elicited cidal activity against L. pneumophila (serogroup 1), with a 4-log decrease in viability within 2 h at 37 ºC. Guinea pig passage of this strain did not affect its sensitivity to LF. Addition of magnesium blocked the bactericidal activity. In addition, human milk was also cidal for L. pneumophila. Salts including CaCl2, Mg(NO3)2, and MgCl2, but not NaCl, blocked killing. Activity was pH dependent with the greatest activity at 5.0. Sensitivity of the organism was markedly affected by the growth conditions. Log-phase 12 h, broth-grown cells were most sensitive, with older cultures appearing more resistant. Plate-grown cells were completely resistant. LF binding, as detected by immunofluorescence microscopy, was temperature dependent (no binding was observed at 4ºC), but was independent of killing (Bortner et al., 1989). Actinobacillus actinomycetemcomitans is a fastidious, facultative Gram-negative rod associated with endocarditis, certain forms of periodontal disease, and other focal infections. Human LF is bactericidal for this pathogen (Kalmar & Arnold, 1988). This cidal activity required an unsaturated (iron- and anion-free) molecule that produced a 2log reduction in viability within 120 min at 37ºC at a concentration of 1.9 µM. Magnesium enhanced LF killing, while other cations, such as potassium and calcium, had no effect. It was reported that selective anions were capable of inhibiting the expression of bactericidal activity by LF on S. mutans 10449 (Lassiter et al., 1987). The ability to block LF expression was directly related to the capacity of the anion to serve as a coordinate ion in iron-binding by the LF molecules. The authors hypothesized the presence of an anionic LF target site on the bacterial surface. Treatment of S. mutans with LF under anaerobic conditions abrogated the bactericidal effect. LF killing could be enhanced with thiocyanate and inhibited by catalase and lactoperoxidase; however, bovine serum albumin was equally effective as an inhibitor. Antimicrobial effects of LF and human milk on Yersinia pseudotuberculosis was reported (Salamah & al-Obaidi, 1995a). Bacterial growth in vitro was inhibited by apobut not holo-LF or human milk. Iron-free human milk and to a lesser extent normal human milk were bactericidal for Y. pseudotuberculosis cells that were suspended in deionized water. The in vivo studies also showed that iron-saturated LF enhanced growth, whereas the viable count was reduced by iron-free LF and EDTA. Nine envelope proteins were decreased or disappeared upon growth in iron-deficient medium, whereas one new high molecular weight protein appeared under the same conditions. The effect of pH, temperature, concentration of magnesium and calcium on the bactericidal activity of LF against Yersinia pseudotuberculosis was investigated (Salamah & al-Obaidi, 1995b). The bactericidal activity of LF was higher at acid pH, whereas the bactericidal activity of TF was higher at alkaline pH. Both were not efficient at 4º, 15º, and 25ºC, but were efficient at 37ºC. LF, but not TF, was very efficient at 42ºC. The activity of both proteins were time and concentration dependent. Calcium did not effect their activity up to 60 mM, whereas magnesium reduced the activity of LF only. C. Adhesion-blockade effect E. coli is one of the major etiological agents of gastrointestinal illnesses in humans and animals. Bacterial adherence to intestinal epithelia is an important step in the pathogenesis of this disease. In the colonization process, bacterial adhesins such as fimbriae may recognize various mammalian subepithelial matrix components as receptors.
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Substances that interfere in this host-pathogen interaction could be of therapeutic and prophylactic value, and nonimmunoglobulin fractions of milk, ileal mucus and mucin are among such potential inhibitors (Holmgren et al., 1981; Miedzobrodzki et al., 1989; Olusanya & Naidu, 1991; Cravito et al., 1991). 1. Adhesion-blockade of enteric pathogens. Several carbohydrates, such as 0.1% fucose or 0.5% glucose, as well as LPS (10 µg/ml) isolated from Shigella flexneri strongly inhibit the adherence of shigellae to guinea pig colonic cells. Fucose-containing peptides from hLF also inhibit the adhesion of S. flexneri to colonic epithelial cells (Izhar et al., 1987) The non-immunoglobulin component of human milk responsible for the inhibition of E. coli cell adhesion (hemagglutination) mediated by colonization factor antigen I (CFA-I) were identified by chromatographic fractionation of human whey proteins (Giugliano et al., 1995). Free secretory component (fSC) and LF were isolated and both compounds inhibited the hemagglutination by E. coli CFA1+. The lowest concentrations of fSC and LF able to inhibit the hemagglutination by E. coli strain TR50/3 CFA1+ were 0.06 mg/ml and 0.1 mg/ml, respectively. Commercial preparations of LF from human milk and TF from human serum also inhibited the hemagglutination, with MIC values of 0.03 mg/ml and 0.4 mg/ml, respectively. Bovine LF mediated inhibition of hemagglutination activity of type 1 fimbriated E. coli has also been reported (Teraguchi et al., 1996). The agglutination reaction was specifically inhibited by glycopeptides derived from bLF or α-methyl-D-mannoside. These observations indicate that the glycans of bLF could serve as receptors for type 1 fimbrial lectin of E. coli. The ability of LF to inhibit in vivo colonization of E. coli has been examined (Naidu et al., unpublished). Infection with E. coli strain F18 was established in streptomycin-treated mice by gastric intubation and bacterial excretion was estimated as colony forming units per gram (CFU/g) feces. The excretion of strain F18 in feces reached a steady-state (108 CFU/g) within 7 days, independent of challenge (dose: 8 x 108 or 103 CFU). Oral administration of bLF (20 mg/ml in 20% sucrose solution) caused a 1- to >3log reduction in CFU/g feces with high and low dosages of strain F18. The bacterial multiplication in vivo was markedly affected during the early 24 hours of infection, reflecting >3-log lower number of bacteria in the feces (2 x 103 CFU/g) than the control group. Oral administration of LF prior to infection reduced fecal excretion of E. coli from mouse intestine. In vitro effects of bLF on the molecular interactions of E. coli with subepithelial matrix proteins were examined. Bovine LF inhibited the binding of 125I-labeled fibronectin, fibrinogen, collagen type-I, collagen type-IV and laminin to bacteria. This inhibitory effect was bLF dose-dependent, and was independent of coexistence (competitive) or preexistence (non-competitive) of bLF with the tissue matrix proteins. In displacement studies with bacteria-matrix protein complexes, bLF dissociated only collagen type-I and laminin interactions. Electron microscopy revealed the loss of type-1, CFA-I and CFA-II fimbria of E. coli grown in broth containing 10 µM LF. The inhibitory affect of LF on fimbrial expression was further confirmed by hemagglutination and yeast cell agglutination. The presence of 10 µM LF in the growth media, however, did not affect the P-fimbriation in E.coli. These data suggest a strong influence of LF on adhesion-colonization properties of E.coli.
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2. Adhesion-blockade of oral pathogens. The influence of LF, salivary proteins (SP) and BSA on the attachment of Streptococcus mutans to hydroxyapatite (HA) was reported (Visca et al., 1989). Sorption of LF, SP, and BSA to HA was dependent on the protein concentration and reached the end-point at about 80 mg of proteins per gram of HA. Similarly, the number of streptococci adsorbed to HA was correlated to the amount of cells available up to at least 107 cells per mg of HA. The adsorption of LF, SP and BSA on HA reduced the number of attaching S. mutans cells. In particular, SP reduced the adsorption of S. mutans by 30%, whereas pre-coating of HA with apo- or iron-saturated LF resulted in a three orders of magnitude reduction of S. mutans adsorption to HA. The potent adherence-inhibiting effect of apo-LF together with its antibacterial activity against S. mutans suggests an important biological significance of these phenomena in the oral cavity. Whole cells of P. intermedia demonstrate a high degree of binding to fibronectin, collagen type I and type IV and laminin, whereas a moderate interaction was detected with fibrinogen. The ability of bLF to affect the interactions of the above proteins with P. intermedia was examined (Alugupalli et al., 1994). In the presence of unlabeled bLF, a dosedependent inhibition of binding was observed with all five proteins tested. Unlabeled bLF also dissociated the bacterial complexes with these proteins. The complexes with laminin or collagen type I were more effectively dissociated than fibronectin or fibrinogen, whereas the interaction with collagen type IV was affected to a lesser extent. A strain-dependent variation in the effect of bLF was observed. The ability of hLF and bLF to inhibit adhesion of A. actinomycetemcomitans and P. intermedia to monolayers of fibroblasts, HEp-2, KB and HeLa cells was reported (Alugupalli & Kalfas, 1995). The inhibitory effect was dose-dependent in the concentration range 0.5-2500 µg/ml and not related to the bacterial growth phase. In the presence of LF, decreased association of bacteria with the cell monolayers was also found by microscopic examination of the preparations. These data suggested a possibility that LF could prevent the establishment of bacteria in periodontal tissues through adhesion-counteracting mechanisms in addition to its bacteriostatic and bactericidal properties. LF also binds to fibroblast monolayers and matrigel, a reconstituted basement membrane, through ionic interactions. The adhesion of A. actinomycetemcomitans to these substrata was mainly dependent on the ionic strength of the environment. P. intermedia and P. nigrescens also adhere to fibroblasts mainly by ionic interactions, while their adhesion to matrigel seems to be mediated by specific mechanisms. Lectin-type interactions were not found involved in the binding of these bacteria to the substrata. Treatment of either A. actinomycetemcomitans or fibroblasts with LF decreased the adhesion in a dose-dependent manner, while LF treatment of matrigel alone had no adhesion-counteracting effect. Adhesion of P. intermedia and P. nigrescens to matrigel was not significantly affected by the ionic strength, but the presence of LF inhibited the adhesion. LF bound to matrigel, P. intermedia and P. nigrescens was rapidly released, while LF bound to A. actinomycetemcomitans and fibroblasts was retained. These findings indicate that LFdependent adhesion-inhibition of A. actinomycetemcomitans, P. intermedia and P. nigrescens to fibroblasts and matrigel could involve binding of LF to both the bacteria and substrata. The decreased adhesion may be due to blocking of both specific adhesin-ligand as well as non-specific charge-dependent interactions (Alugupalli & Kalfas, 1997).
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FIGURE 6. LFcin isolation by reverse-phase HPLC. Bovine LF was hydrolyzed with porcine gastric pepsin at pH 4.0 and the hydrolysate was fractionated on a Pep-S column. Shaded peaks are fractions with antimicrobial activity against E.coli H10407 in a microplate assay [Naidu & Erdei, unpublished data]. The amino acid sequence and the primary structures of bLFcin and hLFcin peptides are shown with basic residues encircled and sequence positions numbered [adapted from Bellamy et al., 1992].
D. Cationic effect LF was found to contain an antimicrobial sequence near its N-terminus, which appears to function by a mechanism distinct from iron chelation. The identified domain contains a high proportion of basic residues, like various other antimicrobial peptides known to target microbial membranes and it appears to be located on the surface of the folded protein allowing its interaction with surface components of microbial cells (Tomita et al., 1994). Hydrolysates prepared by cleavage of bLF with porcine pepsin, cod pepsin, or acid protease from Penicillium duponti showed strong activity against E. coli O111, whereas hydrolysates produced by trypsin, papain, or other neutral proteases were much less active (Tomita et al., 1991). Low molecular weight peptides generated by porcine pepsin cleavage of bLF showed broad-spectrum antibacterial activity, inhibiting the growth of a number of Gram-negative and Gram-positive species, including strains that were resistant to native LF. The antibacterial potency of the hydrolysate was at least eightfold greater than that of undigested LF with all strains tested. The active peptides retained their activity in the presence of added iron, unlike native LF. The effect of the hydrolysate was bactericidal as indicated by a rapid loss of viability of E. coli O111. A single active peptide representing antimicrobial domain was isolated following gastric pepsin cleavage of hLF, and bLF, and sequenced by automated Edman degradation. The antimicrobial sequence was found to consist mainly of a loop of 18 amino acid residues formed by a disulfide bond between cysteine residues 20 and 37 of hLF, or 19 and 36 of bLF (Bellamy et al., 1992). Synthetic analogs of this region similarly exhibited potent antibacterial properties. The active peptide of bLF was more potent than that of hLF having effectiveness against various Gram-negative and Gram-positive bacteria at concentrations between 0.3 µM and 3.0 µM, depending on the target strain. Effect of the isolated domain was lethal causing a rapid loss of colony-forming capability (FIGURE 6).
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Human LF contains a 46 residue sequence named lactoferricin H (hLFcin) responsible for its cationic antimicrobial properties. Synthetic peptides HLT1, corresponding to the loop region of hLFcin (FQWQR-NMRKVRGPPVS) and HLT2, corresponding to its charged portion (FQWQRNMRKVR), exerted significant antibacterial effects against E. coli serotype O111 strains NCTC 8007 and ML35 (Odell et al., 1996). The corresponding sequences in native hLF were shown to adopt a charged helix and hydrophobic tail within the N-lobe remote from the iron binding site. Sequence similarities between LFcin and dermaseptin and magainins suggest that LFcin may act as an amphipathic α-helix. The basic amino acid-rich region of bovine lactoferricin (bLFcin), RRWQWRMKKLG has many basic and hydrophobic amino acid residues. Using chemically synthesized bLFcin and its substituted peptides, the antimicrobial activities of the peptides were tested by determining the minimal inhibitory concentration (MIC) of E. coli and Bacillus subtilis and the disruption of the outer cell membrane of E. coli, and the peptide’s toxicities were assayed by hemolysis (Kang et al., 1996). The short peptide (B3) composed of only 11 residues had similar antimicrobial activities while losing most of the hemolytic activities as compared with the 25 residue-long ones (B1 and B2). The short peptides (B3, B5 and B7) with double arginines at the N-termini had more potent antimicrobial activity than those (B4 and B6) with lysine. However, no antimicrobial and hemolytic activities were found in B8, in which all basic amino acids were substituted with glutamic acid, and in B9, in which all hydrophobic amino acids were substituted with alanine. The circular dichroism (CD) spectra of the short peptides in 30 mM SDS were correlated with their antimicrobial activities. These results suggested that the 11-residue peptide of bLFcin is involved in the interaction with bacterial phospholipid membranes and may play an important role in antimicrobial activity with little or no hemolytic activity. To study the immunochemical and structural properties of bLFcin derived from N-lobe of bLF, monoclonal antibody (mAb) was prepared and the amino acid sequence concerned with binding to mAb identified (Shimazaki et al., 1996). Mice injected with bLFcin showed no production of antibody specific to this peptide, whereas those with bLFcin-KLH conjugate produced anti-bLFcin antibodies. None of the mAb reacted with bLF C-lobe, hLF or hLFcin. By the reactivity of the mAb against the peptides synthesized on cellulose membranes using spots and against chemically modified derivatives of bLFcin, the antigenic determinant was identified to be the sequence ‘QWR’. Furthermore, three peptides with antibacterial activity toward enterotoxigenic E. coli have been purified from a pepsin digest of bLF (Dionysius & Milne, 1997). All peptides were cationic and originated from the N-terminus of the molecule in a region where a bactericidal peptide, bLFcin, had been previously identified. The most potent peptide, peptide I, was almost identical to bLFcin; the sequence corresponded to residues 17 to 42, and the molecular mass was 3195 as determined by mass spectrometry. A second, less active peptide, peptide II, consisted of two sequences, residues 1 to 16 and 43 to 48 (molecular mass of 2673), linked by a single disulfide bond. The third peptide, peptide III, also a disulfide-linked hetero-dimer, corresponded to residues 1 to 48 (molecular mass of 5851), cleaved between residues 42 and 43. Peptides I and II displayed antibacterial activity toward a number of pathogenic and food spoilage microorganisms, and peptide I inhibited the growth of Listeria monocytogenes at concentrations as low as 2 µM. Bacterial growth curves showed that bactericidal effects of peptides I and II were observable with-
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in 30 min of exposure. The results confirmed and extended those of earlier studies suggesting that the bactericidal domain of LF was localized in the N-terminus and did not involve iron-binding sites. However, the antibacterial studies conducted by Hoek and co-workers (1997) indicated that the activity of LFcin is mainly, but not wholly, due to its N-terminal region. Several peptides sharing high sequence homology with bLFcin were generated from bLF with recombinant chymosin. Two peptides were co-purified, one identical to bLFcin and another differing from this cationic peptide by the inclusion of a C-terminal alanine. Two other peptides were copurified from chymosin-hydrolyzed LF, one differing from bLFcin by the inclusion of C-terminal alanyl-leucine and the other being a heterodimer linked by a disulfide bond. These peptides were isolated in a single step from chymosin-hydrolyzed LF by membrane ion-exchange chromatography and were purified by reverse-phase highpressure liquid chromatography (HPLC). They were characterized by N-terminal Edman sequencing, mass spectrometry, and antibacterial activity determination. Pure LFcin, prepared from pepsin-hydrolyzed LF, was purified by standard chromatography techniques. This peptide was analyzed against a number of Gram-positive and Gram-negative bacteria before and after reduction of its disulfide bond or cleavage after its single methionine residue and was found to inhibit the growth of all the test bacteria at a concentration of 8 µM or less. Sub-fragments of LFcin were isolated from reduced and cleaved peptide by reverse-phase HPLC. Sub-fragment 1 (residues 1 to 10) was active against most of the test microorganisms at concentrations of 10 to 50 µM. Sub-fragment 2 (residues 11 to 26) was active against only a few microorganisms at concentrations up to 100 µM. E. Synergistic effect LF in combination with antibodies has powerful bacteriostatic effects in vitro and this phenomenon provides specific protection against many infections. LF appears to be essential for the antimicrobial function of polymorphonuclear leukocytes against Pseudomonas aeruginosa (Bullen, 1981). Ellison et al. (1990) studied the ability of LF and TF to damage the Gram-negative outer membrane. Lipopolysaccharide (LPS) release by the proteins could be blocked by concurrent addition of Ca2+ and Mg2+. Addition of Ca2+ also blocked the ability of LF to increase the susceptibility of E. coli to rifampicin. TF, but not LF, increased susceptibility of Gram-negative bacteria to deoxycholate, with reversal of sensitivity occurring with exposure to Ca2+ or Mg2+. In transmission electron microscopy studies polymyxin B caused finger-like membrane projections, but no morphological alterations were seen in cells exposed to EDTA, LF or TF. These data provide further evidence that LF and TF act as membrane-active agents with the effects modulated by Ca2+ and Mg2+. Antimicrobial activities of LF were tested against 15 strains of 10 species of bacteria, and potent activities against Staphylococcus aureus, E. coli, Klebsiella pneumoniae and Proteus spp. were observed. Concomitant use of LF with antibiotic cefodoxime proxetil resulted in a synergistic activity against S. aureus, E. coli, K. pneumoniae and Pseudomonas aeruginosa; and an additive activity against E. coli strain NIHJ and Providencia rettgeri. The minimum inhibitory concentrations (MICs) of antibiotic in the presence of LF was reduced to < 1/64 with an efficacy rate of 53/57 (92.9%) in a patient group with infections (Chimura et al., 1993).
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FIGURE 7. LF synergism with antibiotic cefuroxime. Growth of S. typhimurium strain ATCC13311 in special peptone yeast extract broth at 37˚C was measured as change in optical density at 540 nm. Bacterial growth in media: control (❍); 500 µg/ml of bLF (❑); 0.25 g/ml cefuroxime ( ) and mixture of both agents at the above concentrations () [from Naidu & Arnold (1994) with permission from Elsevier Science Inc.].
The antibiotic susceptibility of Salmonella sp. in the presence of LF was examined (Naidu & Arnold, 1994). A mixture containing sub-minimum inhibitory concentration levels of LF (MIC/4) and cefuroxime (MIC/2) inhibited the bacterial growth. LF strongly potentiated the action of erythromycin (eight-fold), whereas it increased the activity only by two-fold for ampicillin, ciprofloxacin, chloramphenicol, and rifampicin; similarly, these antibiotics also reduced the MIC of bLF by two-fold in S. typhimurium. Such antimicrobial potentiation was not observed with bLF mixtures containing cefalexin, gentamycin, or polymyxin B against strain ATCC13311. BLF and cefuroxime also demonstrated potentiation of varying degrees (2- to 16-fold) with nine other Salmonella species. These data established the binding of LF to porins in salmonellae and a potentiation effect of LF with certain antibiotics (FIGURE 7). The effects of LF and its peptides in combination with azole antifungal agents against Candida albicans were investigated by a micro-broth-dilution method (Wakabayashi et al., 1996). For pepsin hydrolysate of LF or the LF-derived antimicrobial peptide bLFcin, the concentrations required to inhibit the growth of Candida decreased in the presence of relatively low concentrations of clotrimazole (CTZ). The MIC of all azole antifungal agents tested was reduced by 1/4-1/16 in the presence of a sub-MIC level of each of these LF-related substances. Polyene and fluoropyrimidine antifungal agents did not show such a combined effect with these LF-related substances. The anti-Candida activity of LF or bLFcin in combination with CTZ was shown synergistic by checkerboard analysis. These results indicate that LF-related substances function cooperatively with azole antifungal agents against C. albicans. Effects of apo-LF and lactoperoxidase system (lactoperoxidase, LP/SCN-/H2O2), separately and together, on the viability of Streptococcus mutans (serotype c) in vitro was tested (Soukka et al., 1991). Streptococci were incubated in buffered KCl (pH 5.5) with
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and without the above components at concentrations normally present in human saliva. Both apo-LF and LP-system had a bactericidal effect against S. mutans at low pH. Together they showed an additive, but not a synergistic, antibacterial effect against S. mutans. Apo-LF enhanced the LP enzyme activity but decreased the yield of the antimicrobial component, hypothiocyanite (HOSCN/OSCN-), when incorporated into the reaction mixtures. This decrease, which was most pronounced at low pH, was due to an LPindependent reaction between apo-LF and HOSCN/OSCN-. The effect of an antimicrobial protein, calprotectin, in combination with neutrophils on the growth of C. albicans was investigated (Okutomi et al., 1998). The growth inhibition of C. albicans by murine neutrophils was augmented by the addition of a low concentration of calprotectin prepared from rat peritoneal exudate cells. The concentrations of calprotectin causing 50% inhibition of growth of C. albicans in the absence or presence of neutrophils at an effector-to-target (E/T) ratio of 30 and 60 were estimated to be 0.45, 0.34 and 0.28 U/ml, respectively. The anti-Candida activity of calprotectin was completely inhibited by 2 µM of zinc ion, while it only partially lowered the activity of the combination of calprotectin and neutrophils. LF has strongly inhibited the growth of C. albicans in combination with calprotectin. These results suggest that calprotectin and LF released from neutrophils may cooperate to inhibit the growth of C. albicans at a local lesion of the infection where there is an accumulation of neutrophils. F. Opsonic effect The ability of hLF to stimulate the phagocytic and cytotoxic properties of macrophages was reported (Lima & Kierszenbaum, 1987). Fe-LF molecule was not required to increase the capacity of mouse peritoneal macrophages to take up Trypanosoma cruzi amastigotes, Listeria monocytogenes, or latex particles; it was necessary for LF to enhance intracellular killing of the two microorganisms. Thus, apo-LF, which did not increase macrophage cytotoxicity, after restoration of ferric ions prior to its use in treatments or when ferric citrate was added to the culture medium immediately after apo-LF treatment of the macrophages, does increase macrophage cytotoxicity. In that iron ions cannot be internalized as such, the latter observation suggested that apo-LF had taken up iron while membrane bound and then enhanced killing. Immunofluorescence studies revealed that comparable proportion of macrophage-bound apo-LF or LF at either 20 or 100% iron saturation were without appreciable differences in fluorescence intensity. Therefore, reduced binding of apo-LF compared with LF was not a likely explanation for the lack of effect of apo-LF on macrophage killing. LF did not enhance amastigote killing by macrophage in the presence of the iron chelator deferoxamine. Diethylaminetriaminepentaacetic acid, an iron chelator which is not incorporated into cells, had a similar effect. The iron-binding protein TF did not alter the capacity of macrophage to either take up or kill the amastigote, indicating that the noted LF effects were not shared by all iron-binding proteins. However, prior treatment of macrophages with TF enabled the cells to display a greater parasite killing capacity after apo-LF treatment, suggesting a role for iron in this activity. Among the known life cycle stages of Trypanosoma cruzi only the amastigote form binds LF. This capacity was readily demonstrable by indirect immunofluorescence in amastigotes derived from mice, a mammalian cell culture, or grown in an axenic medium. No LF binding was detectable on trypomastigotes from blood or mammalian cells, insect-derived metacyclics or epimastigotes, or on epimastigotes grown in Warren’s medi-
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um. Serum levels of LF were increased in mice acutely infected with T. cruzi, and amastigotes from the spleens of these animals were found to have the glycoprotein on their surface. The amastigote LF receptor may have biological significance in parasitehost interaction since mononuclear phagocytes also express an LF receptor, and treatment of these cells with LF has been shown to increase their capacities to take up and kill T. cruzi amastigotes in vitro. The LF receptor is the first marker for T. cruzi amastigotes for which a naturally occurring ligand has been described (Lima et al., 1988). LF bound to Streptococcus agalactiae could interfere with the deposition of complement components on the bacterial surface (Rainard, 1993). Pretreatment of streptococci with LF shortened the lag phase preceding the deposition of C3 component on bacteria. The kinetics of C3 deposition was comparable to that obtained by adding antibodies against S. agalactiae to agammaglobulinaemic precolostral calf serum (PCS) heated at 56 °C for 3 min to inactivate the alternative pathway. Accelerated C3 deposition did not occur in the absence of calcium ions. Deposition of C4 on bacteria occurred only when either antibodies or LF were added to PCS. These results demonstrate that the interaction of LF with bacteria activated the classical pathway of complement in the absence of antibodies. The binding of purified C1q to bacteria was promoted in a dose-dependent manner by LF, suggesting that recruitment of classical pathway of complement resulted from the interaction of C1q with LF-adsorbed to the bacterial surface. Phagocytosis of bacteria opsonized with heated PCS (at 56°C for 3 min) and LF was comparable to that occurring in the presence of heated PCS and antibodies. These data suggested that LF was able to substitute for antibodies in order to activate the classical pathway of complement and to opsonize unencapsulated S. agalactiae efficiently.
VI. ANTIMICROBIAL SPECTRUM Both LF-susceptible and -resistant organisms encompass a variety of types including Gram-positive and Gram-negative bacteria, rods and cocci, and aerobes and anaerobes; both DNA and RNA viruses; a variety of yeast as well as fungi; and parasites. Susceptibility depends on similarities in cell surface structure or the mode of LF action against individual organisms. A. Antibacterial activity The antibacterial properties of milk have been observed for a long time. Most of the relevant literature consists of observations that various pathogenic and saprophytic bacteria are killed or their growth temporarily inhibited by cow’s milk. Bacteriostasis was the widely characterized inhibitory mechanism of LF with well-documented data. Over the past three decades, various laboratories have identified LF as a broad-spectrum antimicrobial and reported a variety of inhibitory mechanisms on both Gram-positive and Gramnegative bacteria (TABLE 3). 1. Gram-positive bacteria. In 1967, Reiter and Oram reported the antibacterial effects of LF against Bacillus stearothermophilus and B. subtilis. This study also observed that apo-LF was unable to inactivate bacterial spores but could inhibit their germination. A decade later, Arnold and co-workers (1977) reported cidal activity of LF against Streptococcus mutans and other oral streptococci.
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The occurrence of LF in saliva has initiated many studies on antimicrobial activity against oral streptococci and control of caries. Apo-LF could cause a potent in vitro growth-inhibition of Streptococcus mutans and this effect could be reversed by iron (Visca et al., 1989). Furthermore, LF seems to reduce the adsorption of S.mutans cells to hydroxyapatite. This adherence-inhibiting effect of apo-LF together with bacteriostasis activity towards S. mutans suggests a possible patho-biological significance of caries control in the oral cavity in vivo. However, apo-bLF seems to elicit a low degree antimicrobial effect on mastitis-associated streptococci in bovine mammary secretions (Todhunter et al., 1985). Naidu and co-workers (1990; 1991) have identified specific LF-binding proteins in Staphylococcus aureus isolated from human and animal infections as well as among various species of coagulase-negative staphylococci causing bovine mastitis. Apo-bLF at concentrations of 0.1%-0.4% could convert compact colonies of Staphylococcus haemolyticus transient to diffused in soft agar (Godo et al., 1997). This surface-active property of LF has prevented autoaggregation of cocci in compact ball-like colonies by hydrophobic interaction or trypsin-sensitive proteins. In vivo anti-staphylococcal activity of hLF, bLF and bLF hydrolysate was reported in an experimental mouse model (Bhimani et al., 1999). All the LF preparations demonstrated weak in vitro antibacterial activity while holo-LFs showed no activity. LF-treated mice (1 mg, i.v.) when injected with 106 staphylococci, showed 30-50% reduction in kidney infections, and viable bacterial counts in the kidney decreased 5- to 12-fold. The inhibitory effect was dose-dependent up to 1 mg LF. The LF preparations were effective when given 1 day prior to the bacterial challenge, after which there was no significant effect even at doses up to 5 mg. Apo- and Fesaturated forms of hLF and bLF were all equally effective, while bLF hydrolysate was not protective. Different degrees of iron-saturation did not alter the in vivo antimicrobial property of either native LF preparation. Feeding mice with 2% bLF in drinking water also reduced the kidney infections by 40-60%, and viable bacterial counts, 5-12-fold. Human LF was shown to be bactericidal in vitro for Micrococcus luteus but not for other Micrococcus species (M. radiophilus, M. roseus and M. varians) (de Lillo et al., 1997). A correlation between the binding of LF to the bacterial surface and the antimicrobial action was observed. Viability assays showed that ferric, but not ferrous, salts prevented binding and consequently M. luteus was not killed. The unsaturated form of LF showed a greater affinity than that of the iron-saturated molecule for lipomannan, a lipoglycan present on the cell wall of M. luteus, supporting the role for lipomannan as one of the possible binding sites of LF on M. luteus. Custer and Hansen (1983) found that LF fragments could react with nitrite and cause inhibition of Bacillus cereus spore outgrowth. LF and lysozyme were shown to inhibit the growth of Bacillus stearothermophilus var. calidolactis spores (Carlsson et al., 1989). The growth of Bacillus cereus could be inhibited by LF and this effect could be reversed by the addition of iron (Sato et al., 1999). The growth inhibition was also reversed by the addition of erythrocytes and hemoglobin. B. cereus seems to use heme or heme-protein complex (hemoglobin-haptoglobin and hematin-albumin complexes) as iron sources in iron deficient conditions. Oral administration of bLF with milk has been reported to inhibit various species of clostridia including C. ramosum, C. paraputrificum and C. perfringens in an experimental mouse model (Teraguchi et al., 1995).
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TABLE 3. Inhibitory spectrum of hLF, bLF and LFcins against various bacteria. Bacterial species
Form
Dose
Effect
Reference
Actino. actinomycetemcomitans Aeromonas hydrophila Bacillus cereus Bacillus circulans Bacillus natto IFO3009 Bacillus stearothermophilus Bacillus subtilis Bacillus subtilis ATCC6633 Bifidobacterium longum Corynebacterium diphtheriae Coryne. ammoniagenes Coryne. renale Clostridium innocuum Clostridium perfringens Clostridium paraputrificum Enterococcus faecalis Escherichia coli E386 Escherichia coli Escherichia coli H10407 Escherichia coli IID-861 Escherichia coli HB101 Escherichia coli CL99 Klebsiella pneumoniae Lactobacillus casei Legionella pneumophila Listeria monocytogenes L. monocytogenes NCTC7973 Micrococcus luteus Proteus vulgaris JCM1668T Pseudomonas aeruginosa Ps. aeruginosa IFO3446 Pseudomonas fluorescens Salmonella abony Salmonella dublin Salmonella enteritidis Salmonella hartford Salmonella kentucky Salmonella panama Salmonella pullorum Salmonella rostock Salmonella salford Salmonella montevideo Salmonella thompson Salmonella typhimurium Rd Salm. typhimurium R10 Salm. typhimurium SL696 Salmonella virchow Shigella flexneri Staphylococcus albus Staphylococcus aureus Staph. aureus JCM2151 Staphylococcus epidermidis Staphylococcus haemolyticus Staphylococcus hominis
hLF bLF bLFcin bLFcin bLFcin bLF bLF bLFcin bLF bLFcin bLFcin bLFcin bLF bLFcin bLFcin bLFcin bLF hLF bLF bLFcin hLF bLF bLFcin bLFcin hLF bLFcin bLFcin bLF bLFcin hLF bLFcin bLFcin bLF bLF bLFcin bLF bLF bLF bLF bLF bLFcin bLF bLF bLF bLF bLF bLF bLF bLF bLF bLFcin bLFcin bLFcin bLFcin
2 µM 0.1% 6 µM 0.006% 0.002% 1:20 1:20 0.002% 0.1% 0.018% 0.003% 0.001% 0.1% 0.024% 0.003% 0.06% 0.1% 42 µM 0.1% 10 µM 0.2% 20 µM 10 µM 0.012% 0.03% 10 µM 2 µM 0.1% 0.012% 42 µM 10 µM 8 µM 0.8% 0.2% 0.012% 0.8% 0.2% 0.1% 0.2% 0.2% 4 µM 20 µM 0.1% 0.5% 0.1% 20 µM 0.8% 0.1% 0.5% 0.1% 10 µM 0.006% 0.001% 0.003%
Cidal (2-log reduction) Adhesion-blockade (47%) Cidal (4-log, 100%) Cidal (6-log, 100%) Cidal (6-log, 100%) Stasis Stasis Cidal (6-log, 100%) Agglutination Cidal (6-log, 100%) Cidal (6-log, 100%) Cidal (6-log, 100%) Agglutination Cidal (6-log, 100%) Cidal (6-log, 100%) Cidal (6-log, 100%) Stasis (24-h, 100%) Cidal (6-log reduction) Adhesion-blockade (50%) Cidal (3-log reduction) Invasion-inhibition LPS release, OM damage Cidal (3-log reduction) Cidal (6-log, 100%) Cidal (4-log reduction) Cidal (4-log reduction) Cidal (4-log, 100%) Agglutination Cidal (6-log, 100%) Cidal (7-log, 100%) Cidal (3-log reduction) Cidal (4-log, 100%) Stasis (24-h, 100%) Stasis (24-h, 100%) Cidal (6-log, 100%) Stasis (24-h, 100%) Stasis (24-h, 100%) Stasis (24-h, 100%) Stasis (24-h, 100%) Stasis (24-h, 100%) Cidal (4-log, 100%) LPS release, OM damage Stasis (24-h, 100%) Stasis (64%) Adhesion-blockade (68%) LPS release, OM damage Stasis (24-h, 100%) Adhesion-blockade (30%) Stasis Adhesion-blockade (54%) Cidal (3-log reduction) Cidal (6-log, 100%) Cidal (6-log, 100%) Cidal (6-log, 100%)
Kalmar & Arnold, 1988 Paulsson et al., 1993 Hoek et al., 1997 Bellamy et al., 1992 Bellamy et al., 1992 Reiter & Oram, 1967 Reiter & Oram, 1967 Bellamy et al., 1992 Tomita et al., 1994 Bellamy et al., 1992 Bellamy et al., 1992 Bellamy et al., 1992 Tomita et al., 1994 Bellamy et al., 1992 Bellamy et al., 1992 Bellamy et al., 1992 Naidu et al., 1993 Arnold et al., 1980 Paulsson et al., 1993 Bellamy et al., 1992 Longhi et al., 1993 Yamauchi et al., 1993 Bellamy et al., 1992 Bellamy et al., 1992 Bortner et al., 1986 Bellamy et al., 1992 Hoek et al., 1997 Tomita et al., 1994 Bellamy et al., 1992 Arnold et al., 1980 Bellamy et al., 1992 Hoek et al., 1997 Naidu & Arnold, 1994 Naidu & Arnold, 1994 Bellamy et al., 1992 Naidu & Arnold, 1994 Naidu & Arnold, 1994 Naidu & Arnold, 1994 Naidu & Arnold, 1994 Naidu & Arnold, 1994 Hoek et al., 1997 Yamauchi et al., 1993 Naidu & Arnold, 1994 Naidu et al., 1993 Paulsson et al., 1993 Yamauchi et al., 1993 Naidu & Arnold, 1994 Paulsson et al., 1993 Masson et al., 1966 Paulsson et al., 1993 Bellamy et al., 1992 Bellamy et al., 1992 Bellamy et al., 1992 Bellamy et al., 1992
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Bacterial species
Form
Dose
Effect
Reference
Streptococcus bovis Streptococcus cremoris Streptococcus lactis Streptococcus mitior Streptococcus mutans AHT Strep. mutans LM-7 Strep. mutans ATCC25175 Streptococcus pneumoniae Streptococcus salivarius Streptococcus thermophilus Vibrio cholerae 569B
bLFcin bLFcin bLFcin hLF hLF hLF hLF hLF hLF bLFcin hLF
0.006% 0.003% 0.003% 42 µM 0.17% 42 µM 0.01% 42 µM 83 µM 0.003% 0.33%
Cidal (6-log, 100%) Cidal (6-log, 100%) Cidal (6-log, 100%) Cidal (6-log, 100%) Cidal (7-log, 100%) Cidal (8-log, 100%) Agglutination Cidal (7-log, 100%) Cidal (7-log, 100%) Cidal (6-log, 100%) Cidal (7-log, 100%)
Bellamy et al., 1992 Bellamy et al., 1992 Bellamy et al., 1992 Arnold et al., 1980 Arnold et al., 1977 Arnold et al., 1980 Soukka et al., 1993 Arnold et al., 1980 Arnold et al., 1980 Bellamy et al., 1992 Arnold et al., 1977
Groenink and co-workers (1999) reported a potent antimicrobial activity of synthetic cationic peptides derived from the N-terminal domain that comprises an amphipathic a-helix in hLF (hLF 18-31 and hLF 20-38) and bLF (bLF 17-30 and bLF 19-37). Peptide bLF 17-30, containing the largest number of positively charged amino acids, elicited the highest inhibitory spectrum against both Gram-positive and Gram-negative bacteria. 2. Gram-negative bacteria. Many studies have shown the antimicrobial activity of LF against Gram-negative bacteria, E. coli, in particular. Various antimicrobial effects of LF were demonstrated against E.coli and different mechanisms were postulated to elucidate these effects. LF elicits a bacteriostatic effect on E. coli. Based on the time required for E.coli O111 to reach one-half maximal cell density, Stuart and co-workers (1984) indicated that the in vitro effects of LF on the growth of E. coli was kinetic rather than bacteriostatic. Compared to a control, added apo-LF (0.25-1.0 mg/ml) produced only a delay effect indicating that these concentrations are probably within the sub-inhibitory concentration range. The kinetic delay effect of apo-LF also increased steadily in the presence of Zn2+ and Cu2+ cations. Cu2+, Zn2+ and nitrilotriacetate did not affect the growth rate of this organism in the absence of LF compared to the control. These studies indicate that the mechanism by which LF alters the bacterial growth of E. coli O111 is more complex than simple iron deprivation. Rainard (1987) reported the antibacterial activity of milk against a virulent strain of E. coli using milk fractions from normal or inflamed glands. Whey obtained from mastitis milk exhibited either bactericidal or bacteriostatic activities, depending on whether bacteria were enumerated by the pour plate technique or by surface plating onto sheep blood agar. The cidal activity, however, was not due to LF, even when assayed in distilled water. Milk whey ultra-filtrate was used to assay the ability of normal and mastitis milk to support the antibacterial activities of LF against E. coli. The addition of purified LF to ultra-filtrate from mastitis whey resulted in bacteriostasis, whereas LF was without effect in ultra-filtrate from normal whey. It was suggested that LF could inhibit the growth of LF-sensitive bacteria during mastitis depending on plasma exudation during mastitis. Dionysius et al. (1993) reported that the antibacterial activity of apo-LF depends on bacterial inoculum size and the addition of holo-LF or cytochrome-C could diminish the effect. Furthermore, the resistance to inhibition by LF was not related to the production of bacterial siderophores in E.coli.
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Ellison et al. (1988) hypothesized that the iron-binding proteins could affect the Gram-negative outer membrane in a manner similar to that of the chelator EDTA. Further, both the whole protein and a cationic N-terminus peptide fragment directly damage the outer membrane of Gram-negative bacteria suggesting a mechanism for the supplemental effects. Several groups have also shown that LF could synergistically interact with immunoglobins, complement, and neutrophil cationic proteins against Gram-negative bacteria. Klebanoff and Waltersdorf (1990) found that Fe2+ and apo-LF could generate hydroxy radicals via an H2O2 intermediate with toxicity to E.coli, and hypothesized that such a mechanism could possibly contribute to the microbicidal activity of phagocytes. LF binds to surface structures expressed in E. coli K-12 strains grown under iron limitation (Visca et al., 1990). Both apo and holo forms of LF yielded a maximum of 1.6 X 105 bound molecules/E. coli K-12 cell. The amount of LF bound was independent of the expression of iron-regulated outer membrane proteins. However, LF did not bind to E. coli clinical isolates. Apo-LF (500 µg/ml) in a chemically defined medium inhibited the growth of E. coli K-12 strains but not of clinical isolates. These findings suggested that the antibacterial activity of the protein could be associated to its binding to the cell surface. Enterotoxigenic strains demonstrate higher LF interaction than enteropathogenic, enteroinvasive, enterohemorrhagic strains or normal intestinal E. coli isolates (Naidu et al., 1991). Also the enteropathogenic strains belonging to serotypes O44 and O127 demonstrate higher LF binding compared to O26, O55, O111, O119 and O126 serotypes. No significant differences in the degree of hLF or bLF binding were noticed between aerobactin-producing and non-producing strains. In later studies, Naidu and co-workers have identified and characterized porins in the outer membrane of Gram-negative bacteria as the specific receptors for LF interaction (Tigyi et al., 1992; Naidu et al., 1993; Erdei et al., 1994) Using an in vitro model, Gutteberg and co-workers (1990) reported the early effect of E. coli, Streptococcus agalactiae (group B streptococci, GBS) and recombinant tumor necrosis factor alpha (TNF) on the release of LF and the generation of interleukin1 (IL-1) due to E. coli, using heparinized whole blood from healthy full-term newborns. In a final concentration of 107 per ml both bacteria increased the release of LF markedly. The response to E. coli was immediate. GBS was a less potent stimulant than E. coli and the response was only apparent after 20 minutes. TNF in a concentration of 10 ng/ml as well as 1 ng/ml increased the release of LF significantly, whereas a concentration of 0.1 ng/ml had no effect. Whole blood incubated with different preparations of LF for 20 minutes did not increase the LF levels. No significant changes in IL-1 levels were observed. LF had bacteriostatic but no bactericidal effect on GBS and Streptococcus mutans. Payne et al. (1990) demonstrated that apo-bLF had bacteriostatic activity against four strains of L. monocytogenes and an E.coli at concentrations of 15 to 30 mg/ml, in UHT milk. At 2.5 mg/ml the compound has no activity against S. typhimurium, P. fluorescens and limited activity against E.coli O157:H7 or L. monocytogenes VPHI (Payne et al., 1994). Human LF and free secretory component (fSC) were shown to inhibit the hemagglutination induced by E. coli CFA1+ (Giugliano et al., 1995). The lowest concentrations of purified fSC and hLF to inhibit the hemagglutination by E. coli strain TR50/3 CFA1+ were 0.06 mg/ml and 0.1 mg/ml, respectively.
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TABLE 4: Lactoferrin – Antiviral effects Viral pathogen
Antiviral effect
Reference
Spleen focus forming virus (SFFV) Human influenza virus Human cytomegalovirus (HCMV)
Decreases multiplication Inhibits viral hemagglutination Inhibits infection & replication Inhibits MT4 cell cytopathy Inhibits adsorption & penetration Prevents plaque formation Inhibits MT4 cytopathic effect Inhibits vero cell cytopathy Effects clinical outcome Inhibits viral multiplication Binds E1 and E2 envelope proteins Inhibits HT-29 cell infection
Hangoc et al., 1987 Kawasaki et al., 1993 Hasegawa et al., 1994 Harmsen et al., 1995 Hasegawa et al., 1994 Fujihara & Hayashi, 1995 Harmsen et al., 1995 Marchetti et al., 1996 Sato et al., 1996 Grover et al., 1997 Yi et al., 1997 Superti et al., 1997
Human herpes simplex virus (HSV-1) Human immunodeficiency virus (HIV) Feline immunodeficiency virus (FIV) Respiratory syncytial virus Hepatitis C virus (HCV) Rotavirus
The antimicrobial activities of bLF, and bLFcin against four clinical isolates of enterohemorrhagic E. coli O157:H7 were reported (Shin et al., 1998). The MICs against these isolates were 3 mg/ml for bLF, and 8-10 µg/ml for bLFcin in 1% Bacto-peptone broth. Transmission electron microscopy findings suggested that bLFcin acts on the bacterial surface and affects cytoplasmic contents. Furthermore, bLFcin affected the levels of verotoxins in the culture supernatant fluid of an E. coli O157:H7 strain. The antimicrobial effect of LF against Salmonella typhimurium was tested by measuring conductance changes in the cultivation media by using a Malthus-AT system (Naidu et al., 1993). Conductance measurement studies revealed that the low-LF-binding strain 395MS with smooth LPS was relatively insusceptible to LF, while the high-LFbinding mutant Rd with rough LPS was more susceptible to LF suggesting an LPS shielding of antimicrobial effect. Later studies have led to the identification of porins as LFbinding outer membrane proteins in various species of Salmonellae (Naidu & Arnold, 1994). Antimicrobial effects of LF against various Gram-negative bacterial pathogens, including Aeromonas hydrophila, Yersinia enterocolitica, Campylobacter jejuni, Helicobacteri pylori, Pseudomonas aeruginosa, Vibrio sp., have also been reported (Arnold et al., 1977; Paulsson et al., 1993; Tomita et al., 1994). B. Antiviral activity LF demonstrates a broad-spectrum antiviral activity against both DNA and RNA viruses (TABLE 4). The ability of LF to interact with nucleic acids as well as its capacity to bind eucaryotic cells and prevent viral adhesion seem to be the possible antiviral mechanisms. Abramson et al. (1984) suggested that the depressed chemotactic activity of PMNL infected with influenza virus could be due to changes occurring at the plasma membrane. Virus-treated PMNL stimulated with FMLP or Staphylococcus aureus exhibited a marked decrease for LF released into phagosomes, onto the cells’ outer membrane, and into the extracellular medium as compared to control cells. Baynes et al. (1988) with the use of an immunoperoxidase stain for LF, showed that neutrophils in viral illness have reduced LF content compared to normal subjects. The authors suggested an acquired defect of neutrophil LF synthesis in viral infection. The LF levels in parotid saliva from
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individuals with different clinical stages of human immunodeficiency virus (HIV) infection were significantly decreased in parallel with their markedly reduced parotid secretory IgA output. This combined deficiency of parotid LF and secretory IgA may well contribute to the frequent oral infections seen in subjects with HIV infection (Muller et al, 1992). Purified holo-hLF and recombinant murine IL-3 were assessed in vivo for their effects on replication of Spleen Focus Forming Viruses (SFFV) in spleens of DBA/2 mice injected with the polycythemia-inducing strain of the Friend Virus Complex (FVC) (Hangoc et al, 1987). LF and IL-3, inoculated 2 hr prior to the administration of the polycythemia-inducing strain of the FVC, respectively decreased and increased the replication of SFFV in mice as assessed by the spleen focus forming unit assay in primary and secondary DBA/2 mice. Since virus infectivity is associated with the DNA synthetic phase of the cell cycle and it has been shown that LF decreases and IL-3 increases the percent of hematopoietic progenitor cells in S-phase in vivo, the results suggest that the opposing actions of LF and IL-3 on replication of SFFV may reflect the actions of these molecules on cycling of the target cells for SFFV. Human LF and bLF inhibit the infection of tissue culture cells with human cytomegalovirus (HCMV) and human herpes simplex virus-1 (HSV-1) (Hasegawa et al, 1994). The addition of LF inhibited both in vitro infection and replication of HCMV and HSV-1 in human embryo lung host cells. The maximum inhibition by more than six exponential of ID50 for HCMV and four exponential for HSV-1 was obtained at a concentration in a range from 0.5 to 1 mg of LF per ml of medium. The antiviral activity of LF was associated with its protein moiety, but not with its iron molecule or sialic acid. Furthermore, LF prevented virus adsorption and/or penetration into host cells, indicating an effect on the early events of virus infection. Preincubation of host cells with LF for 5 to 10 min was sufficient to prevent HCMV infection, even when LF was removed after addition of virus. These results suggest that LF possesses a potent antiviral activity and may be useful in preventing HCMV and HSV-1 infection in humans. Native and chemically derivatized proteins purified from serum and milk were assayed in vitro to assess their inhibiting capacity on the cytopathic effect of human immunodeficiency virus (HIV)-1 and human cytomegalovirus (HCMV) on MT4 cells and fibroblasts, respectively (Harmsen et al, 1995). Only native and conformationally intact LF from bovine or human milk, colostrum, or serum could completely block HCMV infection (IC50 = 35-100 µg/mL). Moreover, native LF also inhibited the HIV-1-inducedcytopathic effect (IC50 = 40 µg/mL). When negatively charged groups were added to LF by succinylation, there was a four-fold stronger antiviral effect on HIV-1, but the antiviral potency for HCMV infection decreased. LF likely exerts its effect at the level of virus adsorption or penetration (or both), because after HCMV penetrated fibroblasts, the ongoing infection could not be further inhibited. A number of native and modified milk proteins from bovine or human sources were analyzed for their inhibitory effects on human immunodeficiency virus type 1 (HIV-1) and HIV-2 in vitro in an MT4 cell test system (Swart et al, 1996). The proteins investigated were LF, α-lactalbumin, β-lactoglobulin A, and β-lactoglobulin B. By acylation of the amino function of the lysine residues in the proteins, using anhydrides of succinic acid or cis-aconitic acid, protein derivatives were obtained that all showed a strong antiviral activity against HIV type 1 and/or 2. The in vitro IC50 values of the aconitylated proteins were in the concentration range of 0.3 to 3
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nM. Succinylation or aconitylation of α-lactalbumin and β-lactoglobulin A/B also produced strong anti-HIV-2 activity with IC50 values on the order 500 to 3000 nM. All compounds showed virtually no cytotoxicity at the concentration used. Peptide-scanning studies indicated that the native LF as well as the charged modified proteins strongly binds to the V3 loop of the gp120 envelope protein, with Ka values in the same concentration range as the above-mentioned IC50. Therefore, shielding of this domain, resulting in inhibition of virus-cell fusion and entry of the virus into MT4 cells, may be the likely underlying mechanism of antiviral action. LF prevents herpes simplex virus type-1 (HSV-1) plaque formation in Vero cell monolayer (Fujihara & Hayashi, 1995). Topical administration of 1% LF prior to the virus inoculation suppressed infection on ocular tissue, however it did not inhibit propagation of the virus in the mouse cornea. Marchetti et al. (1996) reported that both hLF and bLF are potent inhibitors of HSV-1 infection, the concentrations required to inhibit the cytopathic effect in Vero cells by 50% being 1.41 µM and 0.12 µM, respectively. Human LF and bLF exerted their activity through the inhibition of adsorption of virions to the cells independently of their iron withholding property showing similar activity in the apo- and iron-saturated form. The binding of [35S]methionine-labelled HSV-1 particles to Vero cells was strongly inhibited when bLF was added during the attachment step. Bovine LF interacts with both Vero cell surfaces and HSV-1 particles, suggesting that the hindrance of cellular receptors and/or of viral attachment proteins may be involved in its antiviral mechanism. The effect of LF on the growth of rotavirus and respiratory syncytial virus in cell culture was investigated (Grover et al., 1997). LF inhibited the growth of respiratory syncytial virus at a concentration tenfold lower than that normally present in human milk. The ability of LF to inhibit influenza virus hemagglutination was also reported (Kawasaki et al., 1993). Hepatitis C virus (HCV) has two envelope proteins, E1 and E2, which form a hetero-oligomer. During dissection of interacting regions of HCV E1 and E2, Yi et al. (1997) found the presence of an interfering compound or compounds in skim milk identified as LF. The bindings of LF to HCV envelope proteins in vitro were confirmed by Western blotting and by the pull-down assay, with immuno-precipitated LF-bound protein A resin. Direct interaction between E2 and LF was proved in vivo, since anti-hLF antibody efficiently immuno-precipitated with secreted and intracellular forms of the E2 protein. The N-terminal loop of LF, the region important for the antibacterial activity, has only a little role in the binding ability to HCV E2 but affected the secretion or stability of LF. Taken together, these results indicate the specific interaction between LF and HCV envelope proteins in vivo and in vitro. Different milk proteins were analyzed for their inhibitory effect on either rotavirus-mediated agglutination of human erythrocytes or rotavirus infection of the human enterocyte-like cell line HT-29 (Superti et al., 1997). Apo- and Fe-LF inhibited the replication of rotavirus in a dose-dependent manner, apo-LF being the most active. It was shown that apo-LF hinders virus attachment to cell receptors since it is able to bind the viral particles and to prevent both rotavirus hemagglutination and viral binding to susceptible cells. Moreover, LF markedly inhibited rotavirus antigen synthesis and yield in HT-29 cells when added during the viral adsorption step or when it was present in the first hours of infection, suggesting that this protein interferes with the early phases of rotavirus infection.
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C. Antifungal activity LF and lysozyme (muramidase), either singly or in combination, are fungicidal in nature and their combined activity is synergistic. Samaranayake and co-workers (1997) examined 20 oral isolates of Candida krusei and 5 isolates of Candida albicans for their susceptibility to human apo-LF and lysozyme, either singly or in combination, using an in vitro assay system. The two species exhibited significant interspecies differences in susceptibility to LF, but not for lysozyme; C. krusei was more sensitive to LF (1.4 times) than C. albicans. Both species revealed significant intraspecies differences in their susceptibility to lysozyme, but not for LF. No synergistic antifungal activity of the two proteins on either Candida species was noted. LF could inhibit the growth of C.albicans in the absence of PMNL, and anti-LF antibodies reversed both this inhibition and the PMNL activation by MP-F2, GM-CSF, and LPS. Furthermore, PMNL may be activated by relevant candidal mannoproteins, and release of LF may add to other antimicrobial mechanisms of PMNL for the control of candidal infections (Palma et al., 1992). Candida albicans was found highly susceptible to inhibition and inactivation by bLFcin, a peptide produced by enzymatic cleavage of bLF (Bellamy et al., 1993). Effective concentrations of the peptide varied within the range of 18 to 150 µg/ml depending on the strain and the culture medium used. Its effect was lethal, causing a rapid loss of colony-forming capability. 14C-labeled bLFcin bound to C. albicans and the rate of binding appeared to be consistent with the rate of killing induced by the peptide. The extent of binding was diminished in the presence of Mg2+ or Ca2+ ions, which acted to reduce its anticandidal effectiveness. Binding occurred optimally at pH 6.0 and killing was maximal near the same pH. Such evidence suggests the lethal effect of bLFcin results from its direct interaction with the cell surface. Cells exposed to bLFcin exhibited profound ultrastructural damage that appeared to reflect its induction of an autolytic response. D. Antiparasitic activity LF could elicit defense against parasitic infections by phagocytic activity in the destruction of amastigotes, an intracellular parasitic form of Trypanosoma cruzi in macrophages. The effect of bLF on the intracellular growth Toxoplasma gondii parasites was examined in murine macrophage and embryonic cells (Tanaka et al., 1996). Co-cultures of host cells with the parasites were supplemented with LF, apo-LF, holo-LF or TF in the culture media for varying periods. The growth activity of intracellular parasites in the host cells was determined by the measurement of selective incorporation of 3H-uracil. Supplement of LF had no effect on the penetration activity of the parasites, while development of intracellular parasites was inhibited linearly in concentration of LF. Supplement of apo-LF and holo-LF, but not TF showed similar effects. These suggest that LF induce the inhibitory effects on the development of intracellular parasites. Pretreatment of LF to the macrophages, however, did not show any inhibitory effects, whereas mouse embryonic cells preincubated with LF suppressed the intracellular growth. Thus, the action of LF to macrophages would be different from that of mouse embryonic cells. The trophozoites of Giardia lamblia could be killed by nonimmune human milk in a time- and concentration-dependent manner. Removal of greater than 99% of the SIgA from milk did not decrease its Giardia-cidal activity. Thus, the killing was not anti-
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body dependent. Studies by Gillin and co-workers (1983) showed that in the presence of milk, trophozoites lost motility, swelled, and lysed. The Giardia-cidal activity may be specific to human milk, since unheated cow and goat milk were virtually devoid of activity. Human and bLFs and their derived N-terminal peptides were giardicidal in vitro (Turchany et al., 1995). Fe3+, but not Fe2+, protected trophozoites from both native LF and peptides, although the latter lack iron-binding sites. Other divalent metal ions protected only against native LF. Log-phase cells were more resistant to killing than stationaryphase cells. These studies suggest that LF, especially in the form of the N-terminal peptides, may be an important nonimmune component of host mucosal defenses against Giardia lamblia.
VII. INFLUENCING FACTORS A. Citrate / bicarbonate ratio The requirement of bicarbonate for formation of the red complex of LF was first pointed out by Blanc and Isliker (1963). In a later study, Masson and Heremans (1968) clearly established the involvement of bicarbonate in the metal-combining properties of LF. It was found that one molecule of bicarbonate (carbon dioxide) is taken up per atom of iron or copper during the formation of the colored LF-metal complex. It was observed that the color development proceeded very slowly when a gas-free sample of apo-LF was exposed to air in the presence of copper ions, whereas it took place instantly when bicarbonate was added. This suggested that the carbon dioxide from the air first had to become converted to bicarbonate ions before its participation in the reaction. Fresh human and bovine milk are bacteriostatic in vitro for certain (milk-sensitive) strains of E. coli. Dolby et al. (1977) reported that the addition of bicarbonate to the test system could potentiate the bacteriostasis which also results in the inhibition of milkresistant strains. The concentration of bicarbonate needed for such an effect is lower for human milk than for cow milk and is reduced even further by the addition of more LF. In vivo studies with infants and data deduced from the ratio of milk-sensitive to milk-resistant strains of E. coli isolated from fecal samples suggested that the neonatal intestinal secretions may contribute to the bacteriostatic activity of their feeds so that (i) in fully breastfed babies all strains of E. coli are inhibited to the same extent; there is no selection on the basis of milk sensitivity and equal numbers of strains resistant and sensitive to milk are found in the feces; (ii) in fully bottle-fed babies E. coli is not inhibited since the milk is non-bacteriostatic and again there is no selection; (iii) in babies fed at the breast but bottle-milk supplemented, only milk-sensitive strains are inhibited; milk-resistant strains are not, and preferentially colonized the large intestines. Undiluted dialyzed milk was not inhibitory because of its low content of LF and the lack of inhibition in undiluted whey is due to the high concentration of citrate in colostral whey (and milk) (Reiter et al., 1975). It was suggested that citrate competes with the iron-binding proteins for iron and makes it available to the bacteria. Addition of bicarbonate, which is required for the binding of iron by LF, can overcome the effect of citrate. Coliform bacteria respond to low-iron environments by production of iron-sequestering agents that compete effectively with apo-LF for free iron. Addition of apo-LF plus citrate could reverse growth inhibition. The molar ratio (citrate to apo-LF) is more important than the absolute concentration of either component. Bishop et al. (1976) found that a ratio of
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75 resulted in 50% growth inhibition, whereas ratios of 300 and greater resulted in less than 10% growth inhibition. These results suggest that the ratio of citrate to LF is important in the nonspecific protection of bovine udder. Inhibition of E.coli by apo-LF (10 mg/ml) was abolished by addition of ferric iron to the assay system, indicating an irondependent nature of apo-LF induced inhibition of bacteria (Nonnecke & Smith, 1984a). Bicarbonate supplementation of the growth system containing apo-LF (1 mg/ml) increased inhibition of three coliform strains by apo-LF. Addition of increasing concentrations of citrate (2.0 mg/ml) to an assay system containing apo-LF (5 mg/ml) resulted in a concomitant reduction of growth inhibition of three coliform strains. These data further indicate a potential relationship between the molar ratio of citrate to LF of the lacteal secretion and its capacity to inhibit coliform strains associated with mastitis. Changes in pH, concentration of serum albumin, immunoglobulin G, citrate, LF, and number of leukocytes in secretions were typical of milk from glands undergoing physiological transitions. Whey from different glands of the same cow differ markedly in their capacity to inhibit growth of coliforms. Bacteriostatic activity of whey increases markedly during the dry period and reaches maximal in whey collected on day-15 of the dry period and at parturition in the subsequent lactation (Nonnecke & Smith, 1984b). Griffiths and Humphreys (1977) conducted a series of experiments to elucidate the importance of bicarbonate and milieu pH in the bacteriostatic activity of LF. At pH 7.4 and in the presence of bicarbonate, human milk and bovine colostrum inhibit the growth of E. coli O111. Adding sufficient iron to saturate the iron-binding capacity of the LF present in the milk or colostrum prevents bacteriostasis. At pH 6.8, neither milk nor colostrum could inhibit E. coli 0111. Adjusting the pH to 7.4 with bicarbonate resulted in the development of bacteriostatic activity. Adjusting the pH to 7.4 with NaOH was ineffective. Dialyzed colostrum and milk inhibited bacterial growth at pH 6.8 in the absence of added bicarbonate; addition of citrate or iron abolished bacteriostasis. The chromatographic elution profile of tyrosyl-tRNA from iron-replete E. coli differs significantly from that of tyrosyl-tRNA from iron-deficient organisms. Examination of the elution profile tyrosyl-tRNA from E. coli 0111 growing in colostrum without added bicarbonate showed that such bacteria were fully replete in iron. The nature of the elution profile of tyrosyltRNA also showed that iron was freely available to the bacteria when citrate was added to dialyzed colostrum but not available in its absence, even at pH 6.8. These data support the idea that the bacteriostatic action of milk and colostrum, due to the combined action of antibody and LF, depends on the addition of bicarbonate to counteract the iron-mobilizing effect of the citrate normally present in these secretions. Thomas and Fell (1985) reported that in lactating cows hormones [oxytocin or ACTH (Synacthen)] affect the citrate and LF concentrations in the direction that would improve the antibacterial properties of milk, but that this was accompanied by adverse effects on milk secretion. However, the extent of the change was not sufficient to produce inhibition of coliform bacteria. B. Milieu pH In order to apply functionally active bLF to food products, the effect of pH on the heat stability of bLF was studied (Saito et al., 1994). Bovine LF was easily denatured to an insoluble state by heat treatment under neutral or alkaline conditions, above pH 6.0. In contrast, it remained soluble after heat treatment under acidic conditions at pH 2.0 to 5.0, and the HPLC pattern of LF heat-treated at pH 4.0 at 100°C for 5 min was the same as that of native bLF. Bovine LF was thermostable at pH 4.0, and could be pasteurized or © 2000 by CRC Press LLC
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sterilized without any significant loss of its physicochemical properties. Bovine LF was hydrolyzed by heat treatment at pH 2.0 to 3.0 at above 100°C, and its iron binding capacity and antigenicity were lost. Acceleration of the autoxidation of Fe(II) by apoTF or apo-LF at acid pH is indicated by the disappearance of Fe(II), the uptake of oxygen, and the binding of iron to TF or LF. The product(s) formed oxidize iodide to an iodinating species and are bactericidal to E. coli (Klebanoff & Waltersdorph, 1990) Toxicity to E. coli by FeSO4 (10 µM) and human apo-TF (100 µg/ml) or apo-hLF (25 µg/ml) was optimal at acid pH (4.5-5.0) and with log-phase organisms. Both the iodinating and bactericidal activities were inhibited by catalase and the hydroxyl radical (OH.) scavenger mannitol, whereas superoxide dismutase was ineffective. NaCl at 0.1 M inhibited bactericidal activity, but had little or no effect on iodination. Iodide increased the bactericidal activity of Fe(II) and apoTF or apoLF. The formation of OH.was suggested by the formation of the OH.spin-trap adduct (5,5dimethyl-1-pyroline N-oxide [DMPO]/OH)., with the spin trap DMPO and the formation of the methyl radical adduct on the further addition of dimethyl sulfoxide. (DMPO/OH).formation was inhibited by catalase, whereas superoxide dismutase had little or no effect. These data suggest that Fe(II) and apoTF or apo-LF can generate OH. via an H2O2 intermediate with toxicity to microorganisms, and raise the possibility that such a mechanism may contribute to the microbicidal activity of phagocytes. Salamah and al-Obaidi (1995b) studied the effect of pH, temperature, magnesium and calcium on the bactericidal activity of LF and TF against Yersinia pseudotuberculosis. The bactericidal activity of LF was higher at acid pH, whereas the bactericidal activity of TF was higher at alkaline pH. Neither was efficient at 4°, 15°, and 25°C, but both were effective at 37°C. LF, but not TF, was very efficient at 42°C. The activity of both were time and concentration dependent. Calcium did not effect their activity up to 60 mM, whereas magnesium reduced the activity of LF only. LF release from the secondary granules of activated PMNs is markedly lower at pH 7.2 than at pH 6.7 or 8.2 (Leblebicioglu et al., 1996). Moreover, phagocytosis of opsonized bacteria is lower at pH 7.2 than at pH 7.7. In addition to these effects on functional activation, extracellular pH influences the magnitude of intracellular Ca2+ mobilization. These findings suggest that the pH of an inflammatory milieu can selectively influence PMN activation, thereby altering the balance between bacteria and the host response. C. Proteases Holo-bLF is more resistant to proteolysis than the apo-form (Brock et al., 1976; 1978). In the trypsin digests of bLF, up to five different fragments with molecular weights ranging from 25-kDa to 53-kDa were detected, with no obvious qualitative difference between digests of holo and apo forms. The susceptibility of apo-bLF to tryptic digestion was only slightly reduced when the protein was complexed with β-lactoglobulin, suggesting that complex-formation is not a mechanism for protecting LF against intestinal degradation. The susceptibility of hLF and bLF to digestion by trypsin and chymotrypsin has been compared (Brines & Brock, 1983). Neither enzyme had much effect on the hLFmediated antimicrobial activity of human milk, and the iron binding capacity of hLF in the milk was only slightly reduced. Both enzymes had only a slight effect on the iron bind-
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ing capacity of purified hLF. In contrast, trypsin destroyed the antimicrobial activity of bovine colostrum, and, in line with earlier studies, appreciably reduced the iron binding capacity of both colostrum and purified apo-bLF. Holo-bLF was more resistant to digestion. The unusual resistance of apo-hLF to proteolysis may reflect an evolutionary development designed to permit its survival in the gut of the infant. Proteolytic hydrolysis of milk proteins in the mammary gland during involution could influence the bio-functionality of LF and other innate defense factors. Aslam and Hurley (1997) examined the activities of plasmin, plasminogen, and plasminogen activator on proteolysis of LF in mammary gland secretions collected during involution. Activities of plasmin, plasminogen, and plasminogen activator were significantly higher on day-7, -14, and -21 of involution than were those on day-7 postcalving. Protein fragments resulting from hydrolysis were detected by SDS-PAGE in samples collected on day-7, -14, and -21 of involution, but few protein fragments were observed in samples collected on day-7 postcalving when plasmin activity was low. Immunoblot analysis showed that a number of peptides observed during involution were generated from α-s-casein (CN), β-CN, κ-CN, or LF. The appearance of peptides from proteins of mammary secretions during early involution was generally correlated with increased plasmin activity. Elevated plasmin activity during mammary involution may be primarily responsible for the observed concurrent hydrolysis of milk proteins in mammary secretions. The ability of periodontal pathogens Porphyromonas gingivalis, Prevotella intermedia and Prevotella nigrescens to degrade LF was reported (de Lillo et al., 1996). Strains of P. gingivalis completely degraded LF in vitro, whereas P. intermedia and P. nigrescens showed only partial degradation. It was suggested that LF binds to a highaffinity receptor on all these bacteria and, particularly in the case of P. gingivalis, is then degraded by cell-associated proteases. This property may provide protection to the cell against the effects of LF in periodontal sites and so is a possible virulence factor in disease. However, there was no association between the ability to degrade LF and whether the strains had originated from healthy or diseased oral sites. Bacterium- and neutrophil-derived proteases have been suggested to contribute to tissue injury at sites of Pseudomonas aeruginosa infection. Pseudomonas elastase cleavage of LF and TF enhances in vitro iron removal from these proteins by the P. aeruginosa siderophore pyoverdin. Britigan et al. (1993) detected TF and LF cleavage products in bronchoalveolar lavage (BAL) samples from 21 of 22 and 20 of 21 cystic fibrosis (CF) patients, respectively. Three of eleven and two of nine BAL samples from individuals with other forms of chronic inflammatory lung disease had TF and LF cleavage products, respectively. Each patient in whom such products were detected was also infected with P. aeruginosa. No such products were detected in normal individuals. These data provide evidence that P. aeruginosa- and/or human-derived protease cleavage of TF and LF occurs in vivo in the airways of individuals with CF and other forms of chronic lung disease, suggesting that this process could contribute to P. aeruginosa-associated lung injury in these patients. The effect of Vibrio cholerae non-O1 protease on LF was studied in relation to bacterial virulence mechanism (Toma et al., 1996). The proteins treated with the protease were analyzed by SDS-PAGE. The protease has cleaved LF into two fragments of 50-kDa and 34-kDa. The N-terminal amino acid sequencing of these fragments revealed that the cleavage site was near the hinge region, between serine 420 and serine 421. This cleav-
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age could affect the transition from open to closed configuration, which is involved in iron binding and release. However, the anti-bacterial activity of LF was not affected by protease treatment. D. Microbial iron acquisition Iron is essential to all microorganisms. The low concentration of free iron in body fluids creates bacteriostatic conditions for many microorganisms and is therefore an important defense factor of the body against invading bacteria. Iron-binding proteins, such as LF, TF, and ferritin, play a central role in human ferrokinetics. These iron-binding proteins also participate in the process of decreasing iron availability for the microorganisms. LF and TF restrict the amount of ionic iron available in body fluids to 10-18 M (Bullen, 1981). They do so by decreasing iron re-utilization. Anemia of inflammation (previously called anemia of chronic disease) is seen in the setting of infectious, inflammatory, and neoplastic diseases. It results, in part, from changes in the intracellular metabolism of iron. Alterations of iron physiology seen in many clinical circumstances make excess iron available to microorganisms, thus enhancing their pathogenicity. Understanding the molecular basis of iron withholding by the human host, both in the absence of and during infection, and that of iron acquisition by microorganisms may provide us with new and innovative antimicrobial agents and vaccines. Pathogenic bacteria have developed several mechanisms for acquiring iron from the host (see reviews: Otto et al., 1992; Crosa, 1989). Siderophore-mediated iron uptake involves the synthesis of low molecular weight iron chelators called siderophores which compete with the host iron-binding glycoproteins LF and TF for iron. Other ways to induce iron uptake, without the mediation of siderophores, are the possession of outer membrane protein receptors that actually recognize the complex of TF or LF with iron, resulting in the internalization of this metal, and the use of heme-compounds released into the circulation after lysis of erythrocytes. Rogers and Synge (1978) reported that enterochelin, an iron transporting compound of E.coli could abolish the bacteriostatic effect of human milk. The bacteriostatic phase in human milk could be abolished by adding sufficient iron to saturate the LF in human milk, and also by adding supernatant from a 24-h milk culture or by adding enterobactin, an enterobacterial iron chelator (Brock et al., 1983). Growth in the presence of enterobactin was even more rapid than in the presence of excess iron. Partial loss of bacteriostatic activity could be achieved by absorbing the milk with bacterial antigens, but no clear correlation with removal of antibodies to O, K, or H antigens was apparent. Many strains of E. coli are able to synthesize two siderophores, aerobactin and enterochelin. Although aerobactin has a dramatically lower affinity for iron than enterochelin, it has been shown to provide a significant selective advantage for bacterial growth in conditions of iron limitation, such as in the body fluids and tissues. Differential regulation of the genetic determinants of the two siderophores resulted in preferential induction of the aerobactin system in the presence of unsaturated levels of TF and LF (Williams & Carbonetti, 1986). Pathogenic Neisseriae have a repertoire of high-affinity iron uptake systems to facilitate acquisition of this essential element in the human host. They possess surface receptor proteins that directly bind the extracellular host iron-binding proteins TF and LF (see review: Schryvers & Stojiljkovic, 1999). Alternatively, they have siderophore recep-
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tors capable of scavenging iron when exogenous siderophores are present. Released intracellular heme iron present in the form of hemoglobin, hemoglobin-haptoglobin or free heme can be used directly as a source of iron for growth through direct binding by specific surface receptors. Although these receptors may vary in complexity and composition, the key protein involved in the transport of iron (as iron, heme or iron-siderophore) across the outer membrane is a TonB-dependent receptor with an overall structure presumably similar to that determined recently for E. coli FhuA or FepA. The receptors are potentially ideal vaccine targets in view of their critical role in survival in the host. Helicobacter pylori is known to be an etiologic agent of gastritis and peptic ulcer disease in humans. Human LF supported full growth of the H. pylori in media lacking other iron sources, but neither human TF, bovine LF, nor hen ovoTF served as a source for iron (Husson et al., 1993). Since hLF is found in significant amounts in human stomach resections with superficial or atrophic gastritis, the iron acquisition system of H. pylori by the hLF receptor system may play a major role in the virulence of H. pylori infection. Most H. pylori strains also seem to produce extracellular siderophores (Illingworth et al., 1993). The ability of malleobactin to mobilize iron from LF and TF was examined in an equilibrium dialysis assay in the absence of bacteria (Yang et al., 1993). Malleobactin was capable of removing iron from both LF and TF at pH values of 7.4, 6.0, and 5.0. However, the levels of iron mobilization were greater for TF than for LF at all the pH values used in the assay. Bordetella bronchiseptica uses a hydroxamate siderophore for removal of iron from LF and TF rather than relying upon a receptor for these host iron-binding proteins (Foster & Dyer, 1993). Moraxella (Branhamella) catarrhalis, a mucosal pathogen closely related to Neisseria species, is a prominent cause of otitis media in young children and lower respiratory tract infections in adults. Campagnari et al. (1994) demonstrated that M. catarrhalis obtains iron from LF and TF and also maintains growth with ferric nitrate in vitro. Furthermore, when M. catarrhalis is grown under iron-limited conditions, the bacteria express new outer membrane proteins that are not detected in membranes of organisms cultured in an iron-rich environment. These iron-repressible proteins may be important for the acquisition and utilization of iron in vivo, which could allow M. catarrhalis to colonize and survive on human mucosal surfaces. Vulnibactin, a siderophore produced by Vibrio vulnificus, has been shown to sequester TF- or LF-bound iron for growth (Okujo et al., 1996). Comparative studies with the strain producing vulnibactin and its exocellular protease-deficient mutant revealed the involvement of the protease in addition to vulnibactin could be effective in the utilization of Fe(III) bound to TF and LF. It appears that the protease causes cleavage of these proteins, thereby making bound iron more accessible to vulnibactin. In response to environmental iron stress, Vibrio cholerae produces the siderophore vibriobactin as well as a number of iron-induced outer membrane proteins (Tashima et al., 1996). Leishmania chagasi, the cause of South American visceral leishmaniasis, requires iron for its growth. Wilson et al. (1994) reported the ability of promastigote forms of L. chagasi to take up 59Fe chelated to either TF or LF, although uptake from 59Fe-LF occurred more rapidly. 59Fe uptake from either 59Fe-TF or 59Fe-LF was inhibited by a 10fold excess of unlabeled holo-LF, holo-TF, apo-LF, apo-TF, or iron nitrilotriacetate but not ferritin or bovine serum albumin. There was no evidence for a role for parasite-derived siderophores or proteolytic cleavage of holo-LF or holo-TF in the acquisition of iron by
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promastigotes. This capacity to utilize several iron sources may contribute to the organism’s ability to survive in the diverse environments it encounters in the insect and mammalian hosts. Gardnerella vaginalis could acquire iron from hLF, but not from hTF (Jarosik et al., 1998). Siderophore production was detected in G. vaginalis strains and SDS-PAGE of the cytoplasmic membrane proteins isolated from G. vaginalis grown under iron-replete and iron-restricted conditions revealed several iron-regulated proteins ranging in molecular mass from 33- to 94-kDa.
VIII. MICROBIAL INTERACTIONS LF could bind to microbial surface via an array of specific and non-specific interactions. Interactions of LF with specific microbial target sites could lead to events either for promoting host defense (microbial elimination) or microbial virulence (iron acquisition by pathogen) (Naidu & Arnold, 1997). This chapter shall focus the role of LF-binding microbial targets in antimicrobial susceptibility. Various LF-binding microbial targets have been listed in TABLE 5. A. LF-binding targets Specific LF-binding targets were identified on a variety of bacterial pathogens. The binding components in most microorganisms were proteins, and a few lectin-type interactions were also reported. 1. Staphylococcus spp. Bovine LF could bind to the following staphylococcal species associated with bovine intramammary infections: S. epidermidis, S. warneri, S. hominis, S. xylosus, S. hyicus, and S. chromogenes (Naidu et al., 1990). The bLF-binding mechanism was specific, with affinity constants (Ka values) ranging between 0.96 mM and 11.9 mM. The numbers of bLF-binding sites per cell, as determined by using Scatchard analysis, were as follows: S. epidermidis, 3,600; S. warneri, 1,900; S. hominis, 4,100; S. xylosus, 4,400; S. hyicus, 6,100; and S. chromogenes, 4,700. The bLF- binding receptors of the six coagulase-negative staphylococcal species demonstrated marked differences in patterns of susceptibility to proteolytic or glycolytic enzyme digestion and to heat or periodate treatment. These data suggest that the bLF-binding components in S. epidermidis and S. warneri are proteins containing glycosidyl residues. In the remaining four species, the proteinaceous nature of the bLF-binding component was evident, but the involvement of glycosidyl residues was not clear. Naidu and co-workers (1991) investigated the hLF binding property of 489 strains of S. aureus isolated from various clinical sources. The hLF binding was common among S. aureus strains associated with furunculosis (94.3%), toxic shock syndrome (94.3%), endocarditis (83.3%) and septicaemia (82.8%) and other (nasal, vaginal or ocular) infections (96.1%). Naidu et al. (1992) also characterized the hLF-staphylococcal interaction in S. aureus strain MAS-89. The binding of 125I-hLF to strain MAS-89 reached saturation in less than 90 min and was maximal between pH 4 and 9. Unlabelled hLF displaced 125I-HLF binding. Various plasma and subepithelial matrix proteins, such as IgG, fibrinogen, fibronectin, collagen and laminin, which are known to interact specifically with S. aureus, did not interfere with hLF binding. The Scatchard plot was non-linear; that
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Sites/cell
Mass
Affinity (Ka)
Reference
Heat-modifiable OMPs Outer membrane proteins / porins Cell surface protein Cell surface protein Surface layer protein Outer membrane proteins (OMPs) Porins Omp-C, Omp-F & Pho-E Lipopolysaccharide Membrane protein Heat-shock protein Outer membrane protein Cell membrane Outer membrane receptor Outer membrane receptor OMP - IroA protein Fimbriae, lectin-type interaction Cell surface protein Outer membrane protein Outer membrane proteins / porins Outer membrane proteins / porins Outer membrane proteins / porins Outer membrane proteins / porins Outer membrane proteins / porins Outer membrane proteins / porins Outer membrane proteins / porins Outer membrane proteins / porins Outer membrane proteins / porins Outer membrane proteins / porins OMPs, porins OMPs, porins Proteoglycan component Cell wall protein Peptidoglycan component Cell wall protein
ND ND ND ND ND 5,400
29-, 16.5-kDa 30-, 40-, 60-kDa 32-kD 27-kD 33-kDa ND 37-kDa
880 /1,800 nM ND ND ND ND 140 nM
Alugupalli et al.,1995 Kishore et al., 1991 Menozzi et al., 1991 Menozzi et al., 1991 Tomita et al., 1998 Naidu et al., 1991 Erdei et al., 1994 Elas-Rochard et al., 1995 Schryver, 1989 Amini et al., 1996 Dhaenens et al., 1997 Tryon & Baseman, 1987 Biswas & Sparling, 1995 Schryver & Morris, 1988 Pettersson et al., 1994 Sojar et al., 1998 Kalfas et al., 1991; 1992 Carnoy et al., 1994 Naidu & Arnold, 1994 Naidu & Arnold, 1994 Naidu & Arnold, 1994 Naidu & Arnold, 1994 Naidu & Arnold, 1994 Naidu & Arnold, 1994 Naidu & Arnold, 1994 Naidu & Arnold, 1994 Naidu & Arnold, 1994 Naidu & Arnold, 1994 Tigyi et al., 1992 Tigyi et al., 1992 Naidu et al., 1992 Naidu et al., 1990 Naidu et al., 1990 Naidu et al., 1990
Mycoplasma pneumoniae Niesseria gonorrhoeae Neisseria meningitidis Porphyromonas gingivalis Prevotella intermedia 4H Pseudomonas aeruginosa Salmonella abony NCTC6017 Salmonella dublin NCTC9676 Salmonella hartford HNCMB10063 Salmonella panama NCTC5774 Salmonella pullorum NCTC5776 Salmonella rostock NCTC5767 Salmonella kentucky NCTC5799 Salmonella thompson NCTC5740 Salmonella typhimurium ATCC13311 Salmonella virchow NCTC 5742 Shigella flexneri M90T Shigella flexneri M90T Staphylococcus aureus MAS89 Staphylococcus chromogenes AD1 Staphylococcus epidermidis AF9 Staphylococcus hominis AF93
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ND ND ND ND 10,000 ND ND ND ND 45,000 ND ND ND ND ND ND ND ND ND ND ND 4,800 5,700 5,700 4,700 3,600 4,100
106-kD, 105-kD 60-kDa 70-kDa ND 103-kD 105-kD ND 62-kDa 48-kD, 25-kD 38-, 35-, 32-kDa 38-kDa 37-, 35-, 25-kDa 37-kDa 38-, 35-kDa 39-kDa 38-, 35-, 33-kDa 38-, 35-, 33-kDa 38-kDa 38-, 35-, 33-kDa 39-, 22-, 16-kDa 39-, 22-, 16-kDa 67-kDa / 62-kDa ND ND ND
4 / 390 nM ND 2,880 nM ND 20 nM ND ND ND ND 550 nM ND ND ND ND ND ND ND ND ND ND ND 690 nM 104 nM 27 nM 2,500 nM 11,900 nM 3,800 nM
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LF-binding cellular target site
bLF/hLF bLF/hLF hLF hLF bLF bLf/hLF bLf/hLF bLf/hLF hLF bLf/hLF hLF hLF hLF hLF hLF hLF bLf/hLF hLF bLF/hLF bLF/hLF bLF/hLF bLF/hLF bLF/hLF bLF/hLF bLF/hLF bLF/hLF bLF/hLF bLF/hLF hLF bLF hLF bLF bLF bLF
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Actinobacillus actinomycetemcomitans Aeromonas hydrophila CCUG14551 Bordetella bronchseptica Bordetella pertussis Clostridium sp. Escherichia coli E34663 Escherichia coli E34663 Escherichia coli O55B5 Haemophilus influenza KC548 Helicobacter pylori
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TABLE 5: Specific binding of LF to various microbial cell surfaces - density, mass, binding-affinity (association constant) of cellular target sites
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Sites/cell
Mass
Affinity (Ka)
Reference
bLF bLF bLF hLF hLF hLF hLF hLF
Cell wall protein Peptidoglycan component Cell wall protein Cell surface proteins Cell surface proteins Cell wall receptor Cell surface receptor Amastigote cell wall
6,100 1,900 4,400 ND ND 170,000 90,000 1,000,000
ND ND ND 50-, 35-kDa 49-, 34-, 29-kDa ND ND ND
960 nM 3,100 nM 3,300 nM ND ND 3,600 nM 1,000 nM ND
Naidu et al., 1990 Naidu et al., 1990 Naidu et al., 1990 Staggs et al., 1994 Staggs et al., 1994 Tachezy et al., 1996 Peterson & Alderete, 1984 Lima & Kierszenbaum, 1985
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LF type
Staphylococcus hyicus AC166 Staphylococcus warneri AF101 Staphylococcus xylosus AG12 Treponema denticola Treponema pallidum Tritrichomonas foetus Trichomonas vaginalis Trypanosoma cruzi
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Microorganism
Lactoferrin
TABLE 5 (CONT.): Specific binding of LF to various microbial cell surfaces - density, mass, binding-affinity (association constant) of cellular target sites
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implied a low affinity (Ka:155 nM) and a high affinity (Ka:270 nM) binding mechanism. About 5,700 hLF-binding sites/cell were estimated. The staphylococcal hLF- binding protein (hLF-BP) was partially susceptible to proteolytic enzymes or periodate treatment and was resistant to glycosidases. An active hLF-BP with an apparent Mr of about 450-kDa was isolated from strain MAS-89 cell lysate by ion- exchange chromatography on Qsepharose. In SDS-PAGE, the reduced hLF-BP was resolved into two components of 67and 62-kDa. The two components demonstrated a positive reaction with hLF-HRPO in a Western blot. These data established a specific receptor for hLF in S. aureus. 2. Streptococcus spp. The exposure of Streptococcus agalactiae to bLF resulted in the binding of this protein to all the 12 strains of bovine origin tested, and also, although to a lesser degree, to the five tested strains of human origin (Rainard, 1992). The binding of LF was slightly affected by cultivation conditions, and appeared to be heat-stable. The binding of biotinylated LF was inhibited by unlabeled-LF but not by BSA. Hammerschmidt et al. (1999) demonstrated specific binding of hLF to Streptococcus pneumoniae. Pretreatment of pneumococci with proteases reduced hLF binding markedly, indicating that the hLf receptor is proteinaceous. Binding assays performed with 63 clinical isolates belonging to different serotypes showed that 88% of the tested isolates interacted with hLF. Scatchard analysis showed the existence of two hLFbinding proteins with dissociation constants of 57 nM and 274 nM. The receptors were purified by affinity chromatography, and internal sequence analysis revealed that one of the S. pneumoniae proteins was homologous to pneumococcal surface protein A (PspA). The function of PspA as an hLF-binding protein was confirmed by the ability of purified PspA to bind hLF and to competitively inhibit hLF binding to pneumococci. S. pneumoniae may use the hLF-PspA interaction to overcome the iron limitation at mucosal surfaces, and this might represent a potential virulence mechanism. 3. Vibrio spp. Binding of LF to non-invasive Vibrio cholerae was reported (Ascencio et al., 1992). Iron-binding glycoproteins such as ferritin, TF, haemoglobin, and myoglobin moderately inhibited the LF interaction with the vibrios. Monosaccharides (Nacetyl glucosamine, mannose, galactose, and fucose), and other glycoproteins such as fetuin and orosomucoid also moderately inhibited the binding. V. cholerae showed a cell surface associated proteolytic activity which cleaved the cell-bound 125I-labeled LF. 4. Helicobacter pylori: The interactions of Helicobacter pylori spiral and coccoid forms with LF was reported by Khin et al. (1996). The coccoid forms of 14 strains of H. pylori showed significant hLF binding (median 26%), found to be specific and was inhibited by unlabeled hLF and bLF. Amini et al. (1996) reported the binding of bLF to a 60-kDa heat shock protein of H. pylori. Binding ability was related to human immunoglobulin G because bLF binding proteins were isolated by extraction of cell surface associated proteins with distilled water, applied on IgG-Sepharose and nickel sulfate chelate affinity chromatography. Binding was demonstrated by Western blot after purified protein was digested with alphachymotrypsin and incubated with peroxidase-labeled bLF. Binding was inhibited by unlabeled bLF, lactose, rhamnose, galactose, and two iron-containing proteins, ferritin and haptoglobin. Carbohydrate moieties of bLF seem to be involved in binding because glycoproteins with similar carbohydrate structures strongly inhibited binding. Scatchard plot
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analysis indicated a binding affinity (Ka) of 2.88 µM. In addition, binding of H. pylori cells to bLF was enhanced when bacteria treated with pepsin or α-chymotrypsin after isolation from iron-restricted and iron-containing media. 5. Oral bacteria. Interaction of LF with Actinobacillus actinomycetemcomitans was reported (Alugupalli et al., 1995). The binding of hLF and bLF reached maximum within 1 h. LF binding to the bacterium was pH-dependent and reversible. Scatchard analysis indicated the existence of two different types of binding sites on the bacterium, one with a high affinity constant (Ka:0.880 µM) and the other with a low affinity (Ka:1.8 µM). Bacteria in the exponential phase of growth showed higher binding than cells in the stationary phase. Bacteria grown in medium containing serum and/or lysed erythrocytes bound LF to a lesser extent. Heat-inactivated serum, lysed erythrocytes and other proteins such as mucin and laminin inhibited LF binding to A. actinomycetemcomitans in a competitive binding assay. SDS-PAGE and Western blot analysis revealed LF-reactive protein bands at 29-kDa and 16.5-kDa in the CE and OM of A. actinomycetemcomitans. The 29kDa band displayed a heat-modifiable LF-reactive form with a molecular weight of 34kDa. Neither proteinase K-treated cell envelope nor LPS of this bacterium showed reactivity with LF. These data suggest a specific LF interaction with OMPs of A. actinomycetemcomitans. A LF-binding protein with an estimated molecular mass of 57-kDa was identified in the cell envelope of Prevotella intermedia by SDS-PAGE and Western- blot analysis (Alugupalli et al., 1994). Peroxidase-labeled bLF and hLF showed similar specific binding to this protein. B. Porins Porins are a well conserved heat-modifiable, pore-forming outer membrane proteins (OMPs) of the family Enterobacteriaceae. Porins are also reported in certain Gramnegative bacteria. Porins exist as trimers in the outer membrane usually surrounded by nine molecules of LPS. Porins are suggested to play an essential role in the transport of various solutes across the Gram-negative OM. Porins also serve as receptors for certain bacteriophages and colicins (see reviews: Lugtenberg & van Alpen, 1983; Nikaido & Vaara, 1985; Nikaido, 1989). Naidu and co-workers have reported the role of porins as LF anchorages in E.coli and other bacterial members of the family Enterobacteriaceae (Kishore et al., 1991; Tigyi et al., 1992; Erdei et al., 1993; Naidu & Arnold, 1994). 1. Escherichia coli. The degrees of hLF and bLF binding in 169 E. coli strains isolated from human intestinal infections, and in an additional 68 strains isolated from healthy individuals, were examined in a 125I-labelled protein binding assay (Naidu et al., 1991). The binding was expressed as a percentage calculated from the total labelled ligand added to bacteria. The hLF and bLF binding to E. coli was in the range 3.7 to 73.4% and 4.8 to 61.6%, respectively. Enterotoxigenic (ETEC) strains demonstrated a significantly higher hLF binding than enteropathogenic (EPEC), enteroinvasive (EIEC), enterohaemorrhagic (EHEC) strains or normal intestinal E. coli isolates. EPEC strains belonging to serotypes O44 and O127 demonstrated significantly higher hLF binding compared to O26, O55, O111, O119 and O126 serotypes. No significant differences in the degree of hLF or bLF binding were found between aerobactin-producing and non-producing strains. The interaction was further characterized in a high LF-binding EPEC strain, E34663 (serotype O127). The binding was stable in the pH range 4.0 to 7.5, did not dissociate in
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the presence of 2M NaCl or 2M urea, and reached saturation within 2-h. Unlabelled hLF and bLF displaced the 125I-hLF binding to E34663 in a dose-dependent manner. Apo- and iron- saturated forms of LF demonstrated similar binding to E34663. Among various unlabelled subepithelial matrix proteins and carbohydrates tested (in 4-log excess) only fibronectin and fibrinogen caused a moderate inhibition of 125I-hLF binding. According to Scatchard plot analysis, 5,400 hLF-binding sites/cell, with an affinity constant (Ka) of 140 nM, were estimated in strain E34663. These data establish the presence of a specific LFbinding mechanism in E. coli. Gado et al. (1991) reported that E. coli with low hLF binding are insusceptible to group A (A, E1, E2, E3, E6, and K) and group B (B, D, Ia, Ib, and V) colicins. Conversely, a spontaneous hLF high-binding variant demonstrated an increased susceptibility to both colicin groups. Colicin-insusceptible E. coli wild-type strains 75ColT, 84ColT, and 981ColT showed a low degree of hLF binding, i.e., 4, 8, and 10%, respectively. The hLF binding capacity was high in the corresponding colicin-susceptible mutants 75ColS (43%), 84ColS (32%), and 981ColS (43%). Furthermore, hLF low- (< 5%) and high- (> 35%) binding E. coli clinical isolates (10 in each category) were tested for susceptibility against 11 colicins. Colicin V susceptibility did not correlate with hLF binding in either categories. However, with the remaining colicins, three distinct hLFbinding, colicin susceptibility patterns were observed; (i) 10 of 10 hLF low-binding strains were colicin insusceptible, (ii) 6 of 10 hLF high-binding strains were also colicin insusceptible, and (iii) the remaining hLF high binders were highly colicin susceptible. Certain proteins in the cell envelope and outer membrane of wild-type H10407 (hLF low binder, colicin insusceptible) showed a lower mobility in SDS-PAGE compared to the corresponding proteins of mutant H10407(LF) (hLF high binder, colicin susceptible). These mobility differences were also associated with hLF-binding proteins in Western blot (ligand blot) analysis. The wild type showed a smooth form of LPS with a distinct ladder of O-chains, compared to the rough LPS of the mutant.
FIGURE 8. LF interaction with porins of E.coli. Outer membrane analyses of wild-type (JF568) and porin-deficient mutants (PC2416 express PhoE only; JF703 express OmpC only; JF701 express OmpF only; and PC2415 express none of the three porins) of E.coli by urea-SDS-PAGE and western blotting with HRPO-labeled bLF [from Erdei et al. (1994) with permission from the American Society for Microbiology].
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Certain strains of E. coli (bacterial whole cells) demonstrate specific interaction with 125I-LF. A band with a mass of approximately 37-kDa, which was reactive with horseradish peroxidase (HRPO)-labeled LF, was identified in the boiled cell envelope and outer membrane preparations of an LF-binding E. coli strain, E34663, and a non-LF-binding strain, HH45, by SDS-PAGE and Western blotting (Erdei et al., 1994). Such a band was not detected in the unboiled native cell envelope and outer membrane preparations. The molecular mass and the property of heat modifiability suggested that the LF-binding proteins were porins. The native trimeric form of porin OmpF isolated from strain B6 and its dissociated monomeric form both reacted with HRPO-labeled LF and with monoclonal antibodies specific for OmpF. Furthermore, by using E. coli constructs with defined porin phenotypes, OmpF and OmpC were identified as the LF-binding proteins by ureaSDS-PAGE and Western blotting and by 125I-LF binding studies with intact bacteria (FIGURE 8). These data established that LF binds to porins, a class of well-conserved molecules common in E. coli and many other Gram-negative bacteria. However, in certain strains of E. coli these pore-forming proteins are shielded from LF interaction. 2. Salmonella spp. Interaction of LF with the CE and OM of Salmonella typhimurium-type strain ATCC13311 was tested by SDS-PAGE and Western-blot analyses (Naidu & Arnold, 1994). The HRPO-labeled bLF and hLF both recognized a heatmodifiable protein with an estimated molecular mass of 38-kDa in the OM. Simultaneous immunoblotting with an antiporin monoclonal antibody specific for a conserved porin domain in members of Enterobacteriaceae confirmed that the LF-binding protein is a porin. Such LF-binding porin proteins (37- to 39-kDa range) were readily detected in nine other common Salmonella species: S. dublin, S. panama, S. rostock, S. abony, S. hartford, S, kentucky, S. pullorum, S. thompson, and S. virchow. The latter six species also demonstrated one to three weak LF-reactive bands of low molecular weight in their CE. 3. Shigella flexneri. Tigyi et al. (1992) reported the interaction of LF with dysentry pathogen, Shigella flexneri. The interaction was specific, and approximately 4,800 hLF binding sites (Ka:690 nM) or approximately 5,700 bLF binding sites (Ka:104 nM) per cell were estimated in strain M90T by a Scatchard plot analysis. The native CE and OM did not reveal LF-binding components in SDS-PAGE. However, after being boiled, the CE and OM preparations showed three distinct horseradish peroxidase-LF reactive bands of about 39-, 22-, and 16-kDa. The 39-kDa component was also reactive to a monoclonal antibody specific for porin (PoI) proteins of members of the family Enterobacteriaceae. The LF binding protein pattern was similar with bLF or hLF, for Crb+ and Crb- strains. The protein-LF complex was dissociable by KSCN or urea and was stable after treatment with NaCl. Variation (loss) in the O chain of LPS markedly enhanced the LF-binding capacity in the isogenic rough strain SFL1070-15 compared with its smooth parent strain, SFL1070. These data establish that LF binds to specific components in the bacterial OM; the heat-modifiable, anti-PoI-reactive, and LPS-associated properties suggested that the LF-binding proteins are porins in S. flexneri. 4. Aeromonas hydrophila. The interaction of LF with Aeromonas hydrophila was tested in a 125I-labeled protein- binding assay (Kishore et al., 1991). The LF binding was characterized in type strain A. hydrophila ssp. hydrophila CCUG 14551. The hLF and
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bLF binding reached a complete saturation within 2 h. Unlabeled hLF and bLF displaced 125I- hLF binding in a dose-dependent manner, and more effectively by the heterologous (1 µg for 50% inhibition) than the homologous (10 µg for 50% inhibition) ligand. Apoand holo-forms of hLF and bLF both inhibited more than 80%, while mucin caused approx. 50% inhibition of the hLF binding. Various other proteins (including TF) or carbohydrates did not block the binding. Two hLF-binding proteins with an estimated molecular masses of 40-kDa and 30-kDa were identified in a boiled-CE preparation, while the unboiled CE demonstrated a short-ladder pattern at the top of the separating gel and a second band at approx. 60-kDa position. These data establish a specific interaction of LF and the LF-binding proteins seem to be porins in A. hydrophila. C. Lipopolysaccharides (LPS) 1. Interactions. LF was reported to bind lipid A and intact LPS of E. coli, Klebsiella pneumoniae, Pseudomonas aeruginosa, Neisseria meningitides and Haemophilus influenzae (Appelmelk et al. 1994). LF binding to LPS was inhibitable by lipid A and polymyxin B but not by KDO (3-deoxy-D-manno-octulosonate), glycoside residues present in the inner core of LPS. Binding of LF to lipid A was saturable, and with an affinity constant of 2 nM. Elass-Rochard et al (1995) reported the presence of two E. coli 055B5 LPS-binding sites on hLF: a high-affinity binding site (Ka:3.6 nM) and a low-affinity binding site (Ka:390 nM). Bovine LF, which shares about 70% amino acid sequence identity with hLF, showed similar interaction with LPS. Human serum TF, which is known to bind LPS, caused only 12% inhibition of hLF-LPS interaction, suggesting different binding domains on LPS. Binding and competitive binding experiments performed with the N-tryptic fragment (residues 4-283), the C-tryptic fragment (residues 284-692) and the N2-glycopeptide (residues 91-255) isolated from hLF have demonstrated that the high-affinity binding site is located in the N-terminal domain I of hLF, and the low-affinity binding site is present in the C-terminal lobe. The inhibition of hLF-LPS interaction by a synthetic octadecapeptide corresponding to residues 20-37 of hLF and bLFcin (residues 17-41), a proteolytic fragment from bLF, revealed the importance of the 28-34 loop region of hLF and the homologous region of bLF for LPS binding. Direct evidence that this amino acid sequence is involved in the high-affinity binding to LPS was demonstrated by assays carried out with EGS-loop hLF, a recombinant hLF mutated at residues 28-34. After differentiation, HL-60 cells showed a twofold increase of LF- binding sites with no difference in the specificity or affinity of LF between pre- and post-differentiated cells (Miyazawa et al, 1991). CD11a, CD11b, and CD11c Ag, which have been associated with specific binding sites for LPS on monocytes/macrophages, were also increased 3to 4-fold after differentiation. With the use of this system, the effect of LPS on LF binding was tested. At 37°C, LPS enhanced LF binding on HL-60 cells, especially after differentiation. Conversely, at 4°C, LPS inhibited LF binding. There was little effect of temperature on LF binding in the absence of LPS. In the presence of polymyxin B sulfate, the enhanced LF binding by LPS was abrogated. In addition, pretreatment with mAbCD11 and/or mAb5D3, which are associated with or directed against candidate LPS receptors reduced LF binding. Cross-linking studies using an iodinated, photoactivatable LPS derivative ([125I] ASD-LPS) demonstrated specific binding of LPS to LF. These data indicated a dichotomous nature of LF binding on monocyte/macrophage-differentiated HL-60 cells;
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FIGURE 9. LFcin effects on E.coli CL99 I-2 cells (TEM: Bars, 50 nm). Bacteria were incubated for 2-h in 1% Bacto-peptone broth (A); or broth containing 0.1 mg/ml of bLFcin for 0-h (B) or 2-h (C). Bacteria exposed to bLFcin show altered cell membrane morphology with the appearance of membrane blisters. After 2-h incubation a large amount of cell debris was present and a number of remaining cells appear to have a clumping or coagulation of cytoplasmic elements in addition to membrane blistering [from Yamauchi et al., (1993) with permission from the American Society for Microbiology].
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one being mediated by specific LF receptors whereas the other is apparently mainly via LPS receptors after formation of an LF-LPS complex. LF could inhibit iron-catalyzed formation of hydroxyl radical in the presence of LPS at pH 7.4 and 4.5 (Cohen et al, 1992). Low concentrations of LPS could prime neutrophils toward enhanced function, such as formation of stimulated superoxide anion. LF inhibited LPS priming of neutrophils if LPS contamination of the protein (provided by commercial suppliers) was first reduced. Inhibition of LPS priming was observed whether apo-LF or Fe-LF was used. Similar inhibition of LPS priming was observed when neutrophils were incubated with other serum proteins (e.g., albumin, apoTF, or iron-saturated TF). These results indicated that LPS should not be expected to affect the free radical biology of LF, which is a crucial physiologic function of this protein. PMN-induced LF could inactivate LPS, thereby blocking the ability of LPS to prime fresh PMNs for enhanced fMLP-triggered release of superoxide (Wang et al, 1995). Neutrophils (106 cells/ml) inactivation of LPS (10 ng/ml) took 30 min in a kinetic fashion. In addition, LF isolated from PMN population also required 30 min to inactivate LPS, indicating inherently slow binding of LF to LPS. Mononuclear cells failed to inactivate LPS under the same conditions. Studies with isotope-labeled LPS showed that inactivated LPS remained in the medium and was not taken up or destroyed by the PMNs during inactivation. Bovine LF was also reported to diminish the inflammatory reactions induced by Mycobacterium bovis (BCG) in a mouse model (Zimecki & Machnicki, 1994). Human LF, bLF and LFcin-B were found to suppress the IL-6 response in a monocytic cell line (THP-1) when stimulated by LPS (Mattsby-Baltzer et al, 1996). The suppression of bLF was similar to or higher than that of hLF. LFcin-B was the strongest inhibitor of the LPSinduced IL-6 response. For hLF, the strongest inhibition was observed when added 15-30 min after the addition of LPS. Addition of LF before the LPS induced an approximately 45% reduction of the IL-6 response. The results suggest an anti-inflammatory activity of hLF, bLF, and bLFcin through their suppressive effects on the cytokine release. 2. LF-induced LPS release - effects on microbial OM permeability. Ellison and co-workers (1988) reported that the iron-binding proteins could damage the gram-negative outer membrane and alter bacterial outer membrane permeability in a manner similar to that of the chelator EDTA. Studies in barbital-acetate buffer showed that EDTA and hLF cause significant release of radio-labeled LPS from a UDP-galactose epimerase-deficient E. coli mutant and from wild-type S. typhimurium strains. The LPS release was blocked by iron saturation of hLF, occurred between pH 6 and 7.5, was comparable for bacterial concentrations from 104 to 107 CFU/ml, and increased with increasing hLF concentrations. Studies using Hanks balanced salt solution lacking calcium and magnesium showed that TF could cause LPS release. Additionally, both hLF and TF increased the antibacterial effect of a sub-inhibitory concentration of rifampin, a drug excluded by the bacterial outer membrane. Bovine LF and LFcin also reported to release intrinsically labeled [3H] LPS from three bacterial strains, E. coli CL99 1-2, S. typhimurium SL696, and Salmonella montevideo SL5222 (Yamauchi et al, 1993). Under most conditions, more LPS are released by LFcin, the peptide fragment than by whole bLF. In the presence of either, LF or LFcin there is increased killing of E. coli CL99 1-2 by lysozyme. Bovine LF and LFcin have the ability to bind to free intrinsically labeled [3H] LPS molecules, similar to hLF. In addition to these effects, whereas bLF was at most bacteriostatic, LFcin demonstrated consistent
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bactericidal activity against gram-negative bacteria. This bactericidal effect is modulated by the cations Ca2+, Mg2+, and Fe3+ but is independent of the osmolarity of the medium. Transmission electron microscopy of bacterial cells exposed to LFcin show the immediate development of electron-dense membrane blisters (FIGURE 9). LF shows synergism with lysozyme; each protein alone is bacteriostatic, however, the mixture elicit a bactericidal effect for strains of E. coli, S. typhimurium, and Vibrio cholerae (Ellison & Giehl, 1991). The cidal activity is dose dependent, blocked by iron saturation of LF, and inhibited by high calcium levels, although LF does not chelate calcium. Growth media conditions inhibit completely or partially the effect of LF and lysozyme; the degree of inhibition correlate with media osmolarity. Dialysis chamber studies indicated that bacterial killing required direct contact with LF, and experiments with purified LPS suggested that this related to direct LPS- binding by the protein. 3. LPS induction of LF production in vivo. When incubated with Salmonella typhimurium LPS at 37°C, human PMN suspended in serum-free buffer releases the specific granule constituent LF into the surrounding medium (Koivuranta-Vaara et al., 1987). Release of LF from PMN vary with the concentration of LPS as well as with the duration of incubation and is not accompanied by significant release of the cytoplasmic enzyme lactate dehydrogenase. LPS-induced release of LF from PMN was augmented significantly when cell suspensions were supplemented with additional monocytes and lymphocytes. Only monocytes, however, secreted significant amounts of LF-releasing activity (in a time- and concentration- dependent manner) when incubated separately with LPS. LFreleasing activity was heat (80°C for 15 min) labile, eluted after chromatography on Sephadex G-100 with an apparent molecular weight of approximately 60-kDa, and was inhibited by antibodies to TNF-α. Thus, LPS-induced noncytotoxic release of LF from human PMN suspended in serum-free buffer is mediated, at least in part, by TNF-α derived from contaminating monocytes. Injection of Salmonella typhimurium or LPS into mice resulted in a dose-dependent increase in plasma LF. Endotoxin challenge of normal and neutropenic mice showed a direct correlation of plasma LF level with the granulocyte count in peripheral blood. Physiological neutropenia did not inhibit the LF release (Sawatzki & Rich, 1989). In vivo studies by Gutteberg et al. (1989) measured the total serum iron, plasma LF and circulating leukocytes in piglets during the early phase of severe gram-negative septicemia and endotoxemia following infusion of LPS or E. coli. Iron dropped significantly during the first 30 min of LPS infusion from a median of 32 mM to 13.4 mM. A similar decrease in serum iron was observed at 120 min after the E. coli infusion. Plasma levels of LF increased significantly 120 min after the LPS infusion (6 mg/L compared to preinfusion value of 0.25 mg/L). After intravenous infusion of E. coli a significant rise of plasma LF was demonstrated in 30 min after bacterial infusion (2.1 mg/L compared to preseptic value of 0.8 mg/L). This increase was accompanied with a significant drop of circulating leukocytes (7.3 x 109/L compared to preinfusion, 17 x 109/L) in the piglets receiving E. coli by intravenous route. However, intraperitoneal inoculaltion of E. coli did not show any significant change of plasma LF. The rapid onset of hyposideremia during endotoxemia and E. coli septicemia appeared to correlate with the release of LF from granulocytes and the clearance of iron-bound LF from blood or peritoneal cavity. LPS-stimulation of heparinized human blood resulted in a significant rise of LF, TNF-α, and thromboplastin
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levels (Gutteberg et al, 1990). LPS induced the secretion of LF from granulocytes; the levels were 2.1 mg/L (in 5 min) and 5.3 mg/L (in 60 min) compared to the control values of 0.2 mg/L and 1.3 mg/L, respectively. Systemic administration of bLF into mice 24 hours prior to intravenous challenge of LPS (50 mg), significantly lowered the serum concentration of TNF-α and IL-6 (Machnicki et al, 1993). Doses of bLF ( 97%) by treatment with heparin-Sepharose. Eight breast-fed infants (2-10 mo; mean age 5 mo) were fed 700 to 1000 g of each milk in a randomized, cross-over design with each child acting as his/her own control. The milk was labeled with 8.6 µM (0.5 mg) of 58Fe and iron absorption was measured by quantifying the incorporation of the isotope into red blood cells 14 d after intake using thermal ionization mass spectrometry. Fractional iron absorption was significantly lower from breast milk than from LF-free breast milk. The geometric mean (range) was 11.8% (3.4-37.4%) for breast milk and 19.8% (8.4-72.8%) for LF-free breast milk. These results do not support a direct role for LF in the enhancement of iron absorption from human milk at this age. In addition, iron absorption (11.8%) from human milk fed over several feeds was lower than that previously reported for single feed studies. D. Physiological functions The germfree, colostrum-deprived, immunologically ‘virgin’ piglet model was used to evaluate the ability of bLF to protect against lethal shock induced by intravenously administered endotoxin (Lee et al., 1998). Piglets were fed bLF or BSA prior to challenge with intravenous E. coli LPS, and temperature, clinical symptoms, and mortality were observed for 48 h following LPS administration. Prefeeding with LF resulted in a significant decrease in piglet mortality compared to feeding with BSA (16.7 versus 73.7% mortality). Protection against the LPS challenge by LF was also correlated with both resistance to induction of hypothermia by endotoxin and an overall increase in wellness, as quantified by a toxicity score developed for these studies. In vitro studies using a flow cytometric assay system demonstrated that LPS binding to porcine monocytes was inhibited by LF in a dose-dependent fashion, suggesting that the mechanism of LF action in vivo may be inhibition of LPS binding to monocytes/ macrophages and, in turn, prevention of induction of monocyte/macrophage-derived inflammatory-toxic cytokines. Antibody to an estrogen inducible mouse uterine protein (Teng et a., 1986) has been used to isolate cDNA to the messenger RNA. Analysis of the deduced primary structure and additional biochemical characterization indicated that the protein is LF. An increase in the level of LF mRNA of at least 300-fold can be induced in the mouse uterus by estrogen (Pentecost & Teng, 1987). Neutrophils can inactivate LPS and block its ability to prime fresh neutrophils for enhanced fMLP-triggered release of superoxide. Wang et al. (1995) showed that the inactivation of LPS by neutrophils was primarily due to LF. A time course for inactivating LPS showed that neutrophils (5 million/ml) took 30 min to inactivate 10 ng/ml LPS. Mononuclear cells could not inactivate LPS under the same conditions. Experiments with radioactive LPS showed that inactivated LPS remained in the medium and was not taken up or destroyed by the neutrophils during inactivation. Inactivated LPS still gelled Limulus lysate and primed monocytes. Cell-free medium from neutrophil suspensions also inactivated LPS. A single LPS-inactivating factor was purified from medium by heparin-agarose chromatography. SDS-PAGE showed a single band at 80-kDa, which was identified as LF by immunoblotting. Anti-LF immunoglobulin G removed the LPS-inactivating activity from purified LF and cell-free medium. Purified neutrophil LF required 30 min to inactivate LPS, indicating inherently slow binding of LF to LPS.
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Burrin et al. (1996) examined the anabolic effect of orally administered bLF on visceral organ growth and protein synthesis in newborn pigs. We studied a total of 18 unsuckled newborn pigs. Pigs were randomly assigned to one of three dietary treatment groups: bottle-fed (10 ml/h) formula, formula containing physiologic levels (1 mg/ml) of added bLF, or colostrum. After 24 h of feeding, the visceral organ protein synthesis in vivo was measured using a flooding dose of [3H]phenylalanine. The visceral organ protein and DNA mass, as well as intestinal hydrolase activities and villus morphology was also measured. Hepatic protein synthesis in pigs fed either formula containing bLF or colostrum was similar and in both groups was significantly higher than in pigs fed formula. Splenic protein synthesis was not significantly different in pigs fed either formula or formula containing bLF, but was significantly higher in colostrum-fed animals. There were no significant differences in small intestinal growth, protein synthesis, or hydrolase activities between newborn pigs fed formula, formula containing bLF, or colostrum. These results indicate that feeding formula containing physiologic concentrations of added bLF could increase hepatic protein synthesis in newborn pigs, suggesting that colostrum-borne LF serves an anabolic function in neonates. Antitumor activity. Yoo et al. (1997) studied the effect of bLF and bLFcin on inhibition of metastasis in murine tumor cells, B16-BL6 melanoma and L5178Y-ML25 lymphoma cells, using experimental and spontaneous metastasis models in syngeneic mice. Subcutaneous (s.c.) administration of apo-bLF (1 mg/mouse) and bLFcin (0.5 mg/mouse) 1 day after tumor inoculation significantly inhibited liver and lung metastasis of L5178Y-ML25 cells. However, apo-hLF and holo-bLF at the dose of 1 mg/mouse failed to inhibit tumor metastasis of L5178Y-ML25 cells. Similarly, the s.c. administration of apo-bLF as well as bLFcin, but not apo-hLF and holo-bLF, 1 day after tumor inoculation resulted in significant inhibition of lung metastasis of B16-BL6 cells in an experimental metastasis model. Furthermore, in vivo analysis for tumor-induced angiogenesis, both apo-bLF and bLFcin inhibited the number of tumor-induced blood vessels and suppressed tumor growth on day 8 after tumor inoculation. However, in a long-term analysis of tumor growth for up to 21 days after tumor inoculation, single administration of apobLF significantly suppressed the growth of B16-BL6 cells throughout the examination period, whereas bLFcin showed inhibitory activity only during the early period (8 days). In spontaneous metastasis of B16-BL6 melanoma cells, multiple administration of both apo-bLF and bLFcin into tumor-bearing mice significantly inhibited lung metastasis produced by B16-BL6 cells, though only apo-bLF exhibited an inhibitory effect on tumor growth at the time of primary tumor amputation (day-21) after tumor inoculation. These data suggest that apo-bLF and bLFcin inhibit tumor metastasis through different mechanisms, and that the inhibitory activity of bLF on tumor metastasis may be related to ironsaturation. The influence of bLF on colon carcinogenesis was investigated in male F344 rats treated with azoxymethane (Sekine et al., 1997a). After three weekly injections of azoxymethane, the animals received 2 or 0.2% bLF for 36 weeks. No effects indicative of toxicity were noted, but significant reduction in both the incidence and number of adenocarcinoma of the large intestine was observed with both doses. Thus, the incidences of adenocarcinoma in the groups receiving 2% and 0.2% bLF were 15% and 25%, respectively, in contrast to the 57.5% control value. These results suggest a possible application for bLF in the chemoprevention of colon cancer. Sekine et al. (1997b) also reported that
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the administration of bLF (2%) and Bifidobacterium longum (3%) significantly decreased the numbers of aberrant crypt foci. Most importantly large size foci composed of four or more crypts were always significantly decreased by 2% bLF. Studies on the natural killer activity of spleen cells demonstrated enhancement by bLF and B. longum in line with the levels of influence on foci induction, indicating a possible role for elevated immune cytotoxicity in the observed inhibition. Iigo et al. (1999) reported that oral administration of bLF and the bLF hydrolysate also demonstrated significant inhibition of lung metastatic colony formation from s.c. implanted tumors without appreciable effects on tumor growth. bLFcin displayed a tendency for inhibition of lung metastasis. On the other hand, bLF did not exert marked anti-metastatic activity in athymic nude mice bearing Co 26Lu, though bLF had a tendency to inhibit the lung metastatic colony formation associated with anti-asialoGM1 antibody treatment. AsialoGM1+ and CD8+ cells in white blood cells were increased after treatment with bLF. In vitro, the viability of Co26Lu-F55 cells was markedly decreased when co-cultured with white blood cells from mice administrated bLF, but recovered on treatment with anti-asialoGM1 antibody or anti-CD8 mAb and complement. The results suggest bLF and related compounds might find application as tools in the control of metastasis and that asialoGM1+ and CD8+ cells in the blood are important for their inhibitory effects.
X. APPLICATIONS The emerging knowledge about diseases and the role of natural foods in lowering the risk of such disease processes, and research efforts to identify and develop nutritionally important supplemental foods have been steadily increasing. Milk contains the widest range of biologically active ingredients. LF is one such bioactive protein present in milk (milk-derived whey or derivatives). It is a complex molecule with a number of potential functional properties (Naidu & Bidlack, 1998). A. Potential additive for food safety Consumption of cow’s milk has been an integral part of human civilization since antiquity. LF is now recognized as a significant constituent of milk, responsible for nutraceutical benefits and innate protection against intestinal illnesses. A vast amount of literature has been published on the prophylactic, therapeutic, and regulatory role of LF in various physiological functions during the past four decades. The following points validates milk LF as a potent natural antimicrobial for food safety. Ultimately, an antimicrobial must be non-toxic to test animals and humans. It is also important that the antimicrobial be metabolized and excreted by the body. In vivo studies have demonstrated that the liver plays a central role in the elimination of LF from plasma. When injected by intravenous route, LF is taken up rapidly by the receptors in the liver reticuloendothelial system. The integrity of the protein moiety of LF is required for its effective uptake by the liver. Histological and cytochemical investigations indicate that sinusoidal and Kupfer cells are responsible for hepatic uptake of LF (Courtoy et al., 1984). Studies with iodinated LF identified parenchymal cells as the prime source of LF catabolizing activity (Ziere et al., 1992). The liver degrades LF with a half-life of 2.7 h (Regoeczi et al., 1985). LF seems to remain associated with the plasmalemma for prolonged periods of time (Ziere et al., 1992) which could be interpreted as a sign of slow
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internalization. However, LF is readily detected in both endosomes and lysosomes as early as 15 min after administration (Regoeczi et al., 1985). LF appears in bile 35 min after intravenous injection (Regoeczi et al., 1994). Water solubility of an antimicrobial agent is probably the most important physical property. Hydrophilic properties are necessary to assure that the antimicrobial agent is soluble in aqueous phase where microbial growth occurs. LF is water-soluble, yet dissolves in a wide range of inorganic as well as organic solvents. Thermal behavior can also directly influence the activity of an antimicrobial agent, especially with its carry-through properties. If the food is heated during processing, a highly volatile agent such as a phenolic compound can be vaporized and lost. Paulsson et al. (1993) examined the heat-induced enthalpy changes in apo- and iron-saturated bLFs by differential scanning calorimetry. Two thermal transitions with varying enthalpies were observed, depending on the iron-binding status of the protein. Iron-saturated LF was more resistant to heat-induced changes than was the apo-LF. Native LF had two transitional peaks and pasteurization affected only the low temperature transition. Iron-saturated LF revealed a single transitional peak that was resistant to denaturation by pasteurization temperatures. Native LFs, both unheated and pasteurized, showed similar antibacterial properties suggesting temperature-resistance of the molecule. The ability of an antimicrobial compound to ionize can alter its biological activity depending on the pH of the food system in which it is used. LF exerts antimicrobial activity at a wide pH range in different ionic milieus. Natural compounds, occurring as the major food components, can also influence activity of an antimicrobial depending on the properties of the antimicrobial and those of the naturally occurring compound. The cationic nature enables LF to interact and complex with other proteins such as casein, α-lactalbumin (Hekman, 1971; Lampreave et al., 1990), lysozyme (Perraudin et al., 1974), and immunoglobulin-A (Watanabe et al., 1984). Various regulatory functions were attributed to such LF complexes. Interactions with acidic polysaccharides (Mann et al., 1994) which are ubiquitous components of cell membranes. The arginine-rich N-terminus of the LF molecule (Mann et al., 1994) allows LF to bind with varying degrees of affinity to almost any cell, as well as to low-density lipoproteins. Knowledge of the mode of action of an antimicrobial and of the ability of the organisms to overcome this mode of action can be helpful in determining the efficiency and usefulness of an antimicrobial. The protective role of LF in host defense against various microbial illnesses has been established (Naidu & Arnold, 1997). This chapter has identified several of the molecular mechanisms related to LF antimicrobial activity. Valid assay methods for antimicrobial agents are essential so that the levels can be easily determined. Various laboratories have developed rapid, sensitive, enzyme-linked immunosorbant assays (ELISA) for quantitation of LF in different biological systems. Shinmoto et al. (1997) reported a highly sensitive competitive ELISA for bLF. Culliere et al. (1997) recently developed a microparticle-enhanced nephlometric immunoassay for LF quantitation. This assay is sensitive (detection limit in reaction mixture, 0.2 mg/L) and can be performed in diluted milk (1/300 in reaction mixtures), excluding any interference or sample pretreatment. It allows the quantification of LF on a large range of concentrations (0.675-21.6 g/L) with accuracy (linear-recovery in dilution-overloading assay) and precision (3-6% variation). A rapid immunoluminometric assay and a non-competitive avidin-biotin immunoassay were also developed for LF quantitation. The LactoCard, a new commercial assay, allows rapid determination of LF concentrations in 10-15 min.
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Model
Test design (Treated/Total)
LF
Dosage
Carrier
Route Reference
Effect on intestinal iron absorption Effect on tissue mineral content Prophylaxis during neutropenia Effect on fecal microflora Iron absorption in the newborn Effect on muscle growth
Mouse Mouse Human Human Monkey Rats
Effect on iron balance Effect on fecal microflora Serum Zn, Fe & ferritin levels Control of M. paratuberculosis Effects on fecal flora Effects on induced pancreatitis Effect on iron balance Effect on iron balance Antitumor activity Bacteriostasis of Clostridium spp. Effect on bacterial translocation Antiviral activity against stomatitis Protein synthesis de novo Inhibition of induced colon tumors Inhibition of induced colon tumors Control of Toxoplasma gondii
Human Human Human Mouse Mouse Human Bovine Bovine Human Mouse Mouse Cats Porcine Rats Rats Mouse
Suckling mice Suckling mice Cancer patients (5/14) Newborn term infants (38/69) Newborn monkeys (6/6) Adult animals (48/80) Neonatal animals (40/60) 3-week old infants (7/16) New born term infants (29/55) New born term infants (28/51) Gnotobiotic mice (8/32) Gnotobiotic mice (5/75) Adult subjects (6/35) New born calves (7/53) 1-week old calves (12/36) Adult cancer patients (7/7) (9/9); (15/25) & (30/40) 5-week old mice (20/30) Cats 5-10 yr. (1/7) (5/12) New born pigs (6/18) 6-wk rats (70/115) 6-wk rats (16/30) (8/15) 8-wk mice (25/30)
bLF bLF hLF bLF bLF bLF bLF bLF bLF bLF bLF bLF bLF bLF bLF bLF bLF bLF bLF bLF bLF bLF LFcin
4 g/L or 50 µM for 4 wks 4 g/L or 50 µM for 4 wks 800 mg/day for 10 d 2.8 g/L for 14 d 1 g/L one time per diet 0.25, 1 or 4 mg/d for 14-d 0.01-0.1 mg/kg b.wt. 1 g/L for 3.5 mo. 0.1 or 1.0 g/L for 3 mo. 0.1 or 1.0 g/L for 5 mo. 2 mg/L for 10 mo. 2 g/L for 14 days 100 mg/kg b. wt./ dose 11.4 g /day for 5 d 5 g/day for 5-10 d 0.7% per day for 6 mo. 0.5 – 2.0% for 7-14 d 0.5 – 2.0% for 7 d 40 mg/kg b.wt for 14 d 1 g/L for 24 h 0.2 to 2.0% for 30 wks 0.2 to 2.0% for 4-13 wks 0.2 g/kg b.wt for 8-d
Milk Milk Capsule Formula Formula Saline Saline Formula Formula Formula Water Formula Saline Colostrum Formula Formula Milk Milk None Formula Diet Diet Saline
Oral Oral Oral Oral Oral S.C. S.C. Oral Oral Oral Oral Oral I.P Oral Oral Oral Oral Oral Oral Oral Oral Oral I.P
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Fransson et al., 1983 Keen et al., 1984 Trumpler et al., 1989 Balmer et al., 1989 Davidson et al., 1990 Byatt et al., 1990 Byatt et al., 1990 Schulz-Lell et al., 1991 Roberts et al., 1992 Chierici et al., 1992 Hamilton & Czuprynski, 1992 Hentges et al., 1992 Koike & Makino, 1993 Kume et al., 1994 Kume et al., 1995 Kennedy et al., 1995 Teraguchi et al., 1995a Teraguchi et al., 1995b Sato et al., 1996 Burrin et al., 1996 Sekine et al., 1997a Sekine et al., 1997b Isamida et al., 1998
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Test parameter
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TABLE 7. In vivo effects of LF - human clinical trials and consumption studies in different experimental animal models.
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XI. SAFETY AND TOLERANCE LF is already used in a wide range of products including infant formulas, sport and functional foods, personal care products, as well as veterinary and feed specialties. In United States, LF is yet to be considered for a GRAS status. On the other hand, LF products have found a niche in various parts of Europe and southeast Asia controlled by the following regulations. A. Legal status In Europe, bLF is manufactured according to the Dairy Hygiene Directive 92/46 of the EC and meets the corresponding requirements. As per the EC regulations, bLF can be added to food for nutritional reasons. However, for allowed use, the relevant food standards should be considered. In Japan, LF concentrates are allowed under number 438 as ‘a substance composed mainly of LF obtained from mammal’s milk’ in food according to the Ministry of Health and Welfare Announcement No.160 of August 10, 1995. According to the Public Code of Food Additives in South Korea, LF concentrates are allowed in food products. No special provisions are laid down. In Taiwan, LF may be used in special nutritional food stuffs under the condition ‘only for supplementing foods with an insufficient nutritional content and may be used in appropriate amounts according to actual requirements’. B. In vivo metabolism and turnover Bennett and Kokocinski (1979) measured the turnover of 125I-LF in ten adult human subjects by simultaneous organ radioactivity counting procedure. Ferrokinetic studies were performed in three adults after the intravenous injection of [59Fe]LF. 3. LF was rapidly eliminated from the plasma with a mean fractional catabolic rate of 5.7/day. Apo-LF (one subject) was eliminated at a slower rate (fractional catabolic rate 1.22/day). Of the administered 125I label 99% was recovered in the urine, as free iodine, within the first 24 h. In the 59Fe studies no appreciable activity was found in the urine. Organ radioactivity counting showed that LF was rapidly taken up by the liver and spleen. In the 125I studies the rapid excretion of free 125I suggested catabolism at these sites. In the 59Fe studies, the radioactivity persisted in the liver and spleen for several weeks and was slowly transferred to the bone marrow before appearing in circulating erythrocytes. From the values of fractional catabolic rate, plasma LF, neutrophil LF and plasma volume, a ‘derived neutrophil turnover’ was calculated for each subject. The mean value was 8 x 108 neutrophils/day. This is about 1% the value obtained from the actual measurement of labeled cells. It is postulated that this ‘derived value’ represents only that portion of neutrophil turnover accounted for by intravascular senescence. Ziere et al. (1992) characterized the hepatic recognition of LF. Intravenously injected 125I-LF was cleared rapidly from the circulation by the liver (93% of the dose at 5 min after injection). Parenchymal cells contained 97% of the hepatic radioactivity. Internalization, monitored by measuring the release of liver-associated radioactivity by the polysaccharide fucoidin, occurred slowly. Only about 40% of the liver-associated LF was internalized at 10 min after injection, and it took 180 min to internalize 90%. Subcellular fractionation indicated that internalized LF is transported to the lysosomes.
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Binding of LF to isolated parenchymal liver cells was saturable with a dissociation constant of 10 µM (20 x 106 binding sites/cell). Regoeczi et al. (1994) studied the ability of liver to transfer LF from the plasma to the bile by injecting a dose (10 to 20 µg/100 gm) of labeled bLF intravenously and following its appearance in bile over 3 h. Both diferric- and apo-LF peaked in the bile 35 min after administration (i.e., the same time as bovine lactoperoxidase and diferric rat TF). However, only a small portion of the LF dose (approximately 1%) was recovered with the bile in 3 h. On the basis of autoradiographic evidence, the excreted LF appeared intact. The biliary excretion profile of albumin, a protein thought to reach the canaliculus by para-cellular diffusion, was notably devoid of a peak. This, together with competition observed between LF and lactoperoxidase on one hand and diferrin-TF and LF on the other for transfer to bile, suggests that LF is routed through the hepatocyte in vesicles. The process is initiated by binding to a plasma membrane component to which lactoperoxidase and diferric-TF can also bind. Most 59Fe bound to LF accompanied the protein carrier to the bile. The study concluded that under normal circumstances (i.e., when concentration of LF in the plasma is very low), LF transferred from plasma by the liver is probably not the major source of this protein in bile. C. Consumption studies and safety data The in vivo efficacy as well as safety of LF has been documented in human clinical trials and in several consumption studies in experimental animal models (TABLE 7). Infant food formulae have been supplemented with bLF in four different clinical trials at levels of 0.1 to 1.0 g/L for three to five months and at 2.8 g/L for fourteen days to term human infants with no adverse effects. Also, bLF has been safety administered orally to cancer patients at 1.6 g/day for six months. Much higher levels of bLF have been administered orally to mice and rats, as high as 20 g/L of milk for fourteen days and 20 g/kg diet for thirty weeks, respectively, with no known side effects. Subcutaneous or intraperitoneal administration of bLF also support the safety of bLF when it is given by more sensitive routes of delivery. Bovine LF has been given as a single intraperitoneal dose to rats at 100 mg/kg body weight with no known adverse effect. Other animal species, including cats, pigs, calves, and monkeys have been given bLF orally with no detrimental effects. Bovine LF demonstrates structural homology and functional similarity to hLF. However, cow milk contains only about one-tenth the amount of LF compared to its occurrence in human milk. The levels of hLF in colostrum and mature milk is about 30 g/L and 2 g/L. Thus, a safe upper level of LF consumption by children, adolescents, and adults would be expected at these levels. The literature describes no reports on toxicity of LF. No standard toxicology tests (acute, subchronic, chronic, carcinogenicity, reproductive, developmental, etc.) of LF were reported, Furthermore, LF has not been assigned a Chemical Abstract Services (CAS) registry number.
XII. SUMMARY LF is an antimicrobial glycoprotein present in milk and various exocrine secretions that bathe the mucosal surfaces. This metal-binding protein is a multifunctional bioactive molecule with a critical role in many important physiological pathways. LF could © 2000 by CRC Press LLC
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elicit a variety of inhibitory effects against microorganisms comprising stasis, cidal, adhesion-blockade, cationic, synergistic and opsonic mechanisms. Broad-spectrum activity against different bacteria, viruses, fungi and parasites, in combination with anti-inflammatory and immunomodulatory properties makes LF a potent innate host defense mechanism. The current global production of bovine milk LF is approximately 100 metric tons and this figure is continuously increasing. This protein is finding it applications as an active ingredient in infant formulae, and health foods in South-East Asian countries, in particular. LF is also in use as a therapeutic and prophylactic agent to control intestinal illnesses and mucosal infections. Certain oral hygiene products, skin care products, and animal feed supplements contain LF. Recent advances in LF research to elucidate the structural function relationships, antimicrobial mechanisms, cost-effective technologies for large-scale protein isolation and biotechnology is opening unlimited opportunities for this natural antimicrobial in the development of new products and formulation. A number of efficacy studies and clinical trials are ongoing in various laboratories with over 100 patents filed on this molecule in the past 10 years. Undoubtedly, LF is emerging as one of the leading natural microbial blocking agent in food safety and preservation.
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320. Staggs, T.M., Greer, M.K., Baseman, J.B., Holt, S.C., and Tyron, V.V. 1994. Identification of lactoferrinbinding proteins from Treponema pallidum subspecies pallidum and Treponema denticola. Mol. Microbiol. 12:613-619. 321. Stuart, J., Norrell, S., and Harrington, J.P. 1984. Kinetic effect of human lactoferrin on the growth of Escherichia coli 0111. Int. J. Biochem. 16:1043-1047. 322. Superti, F., Ammendolia, M.G., Valenti, P., and Seganti, L. 1997. Antirotaviral activity of milk proteins: lactoferrin prevents rotavirus infection in the enterocyte-like cell line HT-29. Med. Microbiol. Immunol. (Berl.) 186: 83323. Swart, P.J., Kuipers, M.E., Smit, C., Pauwels, R., deBethune, M.P., de Clercq, E., Meijer, D.K., and Huisman, J.G. 1996. Antiviral effects of milk proteins: acylation results in polyanionic compounds with potent activity against human immunodeficiency virus types 1 and 2 in vitro. AIDS Res. Hum. Retroviruses. 12:769-775. 324. Szuchet-Derechin, S., and Johnson, P. 1965. The ‘Albumin’ fraction of bovine milk-II. The isolation and physicochemical properties of the red proteins. Eur. Polymer J. 1:283-291. 325. Tabak, L., Mandel, I.D., Herrera, M., and Baurmash, H. 1978. Changes in lactoferrin and other proteins in a case of chronic recurrent parotitis. J. Oral Path. 1:97-99. 326. Tachezy, J., Kulda, J., Bahnikova, I., Suchan, P., Razga, J., and Schrevel, J. 1996. Tritrichomonas foetus: iron acquisition from lactoferrin and transferrin. Exp. Parasitol. 83:216-228. 327. Tanaka, T., Omata, Y., Saito, A., Shimazaki, K., Igarashi, I., and Suzuki, N. 1996. Growth inhibitory effects of bovine lactoferrin to Toxoplasma gondii parasites in murine somatic cells. J. Vet. Med. Sci. 58: 61-65. 328. Tashima, K.T., Carroll, P.A., Rogers, M.B., and Calderwood, S.B. 1996. Relative importance of three ironregulated outer membrane proteins for in vivo growth of Vibrio cholerae. Infect. Immun. 64:1756-1761. 329. Teng, C. T., Walker, M. P., Bhattacharyya, S. N., Klapper, D. G., DiAugustine, R. P., and McLachlan, J. A. 1986. Purification and properties of an oestrogen-stimulated mouse uterine glycoprotein (approx. 70 kDa). Biochem. J. 240:413-422. 330. Teraguchi, S., Shin, K., Ozawa, K., Nakamura, S., Fukuwatari, Y., Tsuyuki, S., Namihira, H., and Shimamura, S. 1995a. Bacteriostatic effect of orally administered bovine lactoferrin on proliferation of Clostridium species in the gut of mice fed bovine milk. Appl. Environ. Microbiol. 61:501-506. 331. Teraguchi, S., Shin, K., Ogata, T., Kingaku, M., Kaino, A., Miyauchi, H., Fukuwatari, Y., and Shimamura, S. 1995b. Orally administered bovine lactoferrin inhibits bacterial translocation in mice fed bovine milk. Appl. Environ. Microbiol. 61:4131-4134. 332. Teraguchi, S., Shin, K., Fukuwatari, Y., and Shimamura, S. 1996. Glycans of bovine lactoferrin function as receptors for the type 1 fimbrial lectin of Escherichia coli. Infect. Immun. 64:1075-1077. 333. Teuwissen, B., Masson, P.L., Osinski, P., and Heremans, J.F. 1972. Metal-combining properties of human lactoferrin. The possible involvement of tyrosyl residues in the binding sites. Spectrophotometric titration. Eur. J. Biochem. 31:239-245. 334. Thomas, A.S., and Fell, L.R. 1985. Effect of ACTH and oxytocin treatment on lactoferrin and citrate in cows’ milk. J. Dairy Res. 52:379-389. 335. Tigyi, Z., Kishore, A.R., Maeland, J.A., Forsgren, A., and Naidu, A.S. 1992. Lactoferrin-binding proteins in Shigella flexneri. Infect. Immun. 60:2619-2626. 336. Todhunter, D.A., Smith, K.L., and Schoenberger, P.S. 1985. In vitro growth of mastitis-associated streptococci in bovine mammary secretions. J. Dairy Sci. 68:2337-2346. 337. Toma, C., Honma, Y., and Iwanaga, M. 1996. Effect of Vibrio cholerae non-O1 protease on lysozyme, lactoferrin and secretory immunoglobulin A. FEMS Microbiol. Lett. 135:143-147. 338. Tomita, M., Bellamy, W., Takase, M., Yamauchi, K., Wakabayashi, H., and Kawase, K. 1991. Potent antibacterial peptides generated by pepsin digestion of bovine lactoferrin. J. Dairy Sci. 74:4137-4142. 339. Tomita, M., Takase, M., Wakabayashi, H., and Bellamy, W. 1994. Antimicrobial peptides of lactoferrin. Adv. Exp. Med. Biol. 357: 209-218. 340. Tomita, S., Shirasaki, N., Hayashizaki, H., Matsuyama, J., Benno, Y., and Kiyosawa, I. 1998. Binding characteristics of bovine lactoferrin to the cell surface of Clostridium species and identification of the lactoferrin-binding protein. Biosci. Biotechnol. Biochem. 62:1476-1482. 341. Tourville, D.R., S.S. Ogra, J. Lippes, and T.B. Tomassi Jr. 1970. The human female reproductive tract:immunohistological localization of gammaA, gammaG, gammaM “secretory piece” and lactoferrin. Am. J. Obstet. Gynecol. 108:1102342. Trumpler, U., Straub, P.W., and Rosenmund, A. 1989. Antibacterial prophylaxis with lactoferrin in neutropenic patients. Eur. J. Clin. Microbiol. Infect. Dis. 8:310-313. 343. Tryon, V.V., and Baseman, J.B. 1987. 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344. Tsuji, S., Y. Hirata, and K. Matsuoka. 1989. Two apparent molecular forms of bovine lactoferrin. J. Dairy Sci. 72:1130-1136. 345. Tuccari, G., and G. Barresi. 1985. Immunohistochemical demonstration of lactoferrin in follicular adenomas and thyroid carcinomas. Virchows Arch. A. 406:67-74. 346. Tuccari, G., Barresi, G., Arena, F., and Inferrera, C. 1989. Immunocytochemical detection of lactoferrin in human gastric carcinomas and adenomas. Arch. Pathol. Lab. Med.113:912-915. 347. Turchany, J.M., Aley, S.B., and Gillin, F.D. 1995. Giardicidal activity of lactoferrin and N-terminal peptides. Infect. Immun. 63:4550-4552. 348. van Berkel, P.H., Geerts, M.E., van Veen, H.A., Mericskay, M., de Boer, H.A., and Nuijens, J.H..1997.Nterminal stretch Arg2, Arg3, Arg4 and Arg5 of human lactoferrin is essential for binding to heparin, bacterial lipopolysaccharide, human lysozyme and DNA. Biochem. J. 15:145-451. 349. Van Halbeck, H., Dorland, L., Vliegenthar, J.F.G., Spil, G., Cheron, A., and Montreuil, J. 1981. Structure determination of two oligomannoside-type glycopeptides obtained from bovine lactotransferrin, by 500 MHz 1H-NMR spectroscopy. Biochim. Biophys. Acta 675:293-296. 350. Van Snick, J., Masson, P.L., and Heremans, J.F. 1974. The involvement of lactoferrin in the hyposideremia of acute inflammation. J. Exp. Med. 140:1068-1084. 351. Van Snick, J., and Masson, P.L. 1976. The binding of human lactoferrin to mouse peritoneal cells. J. Exp. Med. 144:1568-1580. 352. Visca, P., Berlutti, F., Vittorioso, P., Dalmastri, C., Thaller, M.C., and Valenti, P. 1989. Growth and adsorption of Streptococcus mutans 6715-13 to hydroxyapatite in the presence of lactoferrin. Med. Microbiol. Immunol. (Berl) 178:69-79. 353. Visca, P., Dalmastri, C., Verzili, D., Antonini, G., Chiancone, E., Valenti, P. 1990. Interaction of lactoferrin with Escherichia coli cells and correlation with antibacterial activity. Med. Microbiol. Immunol. (Berl) 179:323-333. 354. Wada, T., Aiba, Y., Shimizu, K., Takagi, A., Miwa, T., and Koga, Y. 1999. The therapeutic effect of bovine lactoferrin in the host infected with Helicobacter pylori. Scand. J. Gastroenterol. 34:238-243. 355. Wakabayashi, H., Abe, S., Okutomi, T., Tansho, S., Kawase, K., and Yamaguchi, H. 1996. Cooperative anti-Candida effects of lactoferrin or its peptides in combination with azole antifungal agents. Microbiol. Immunol. 40:821-825. 356. Wang, C.S., Chan, W.Y., and Kloer, U.H. 1984. Comparative studies on the chemical and immunochemical properties of human milk, human pancreatic juice and bovine milk lactoferrin. Comp. Biochem. Physiol. (B) 78:575-580. 357. Wang, D., Pabst, K.M., Aida, Y., and Pabst, M.J. 1995. Lipopolysaccharide-inactivating activity of neutrophils is due to lactoferrin. J. Leukoc. Biol. 57:865-874. 358. Watanabe, T., Nagura, H., Watanabe, K., and Brown, W.R. 1984. The binding of human milk lactoferrin to immunoglobulin A. FEBS Lett. 168:203-207. 359. Weinberg, E.D. 1975. Nutritional immunity. Host’s attempt to withold iron from microbial invaders. JAMA. 231 (1): 39-41. 360. Wichmann, L., Vaalasti, A., Vaalasti, T., and Tuohimaa, P. 1989. Localization of lactoferrin in the male reproductive tract. Int. J. Androl. 12:179-186. 361. Williams, P.H., and Carbonetti, N.H. 1986. Iron, siderophores, and the pursuit of virulence: independence of the aerobactin and enterochelin iron uptake systems in Escherichia coli. Infect. Immun. 51:942-947. 362. Wilson, M.E., Vorhies, R.W., Andersen, K.A., and Britigan, B.E. 1994. Acquisition of iron from transferrin and lactoferrin by the protozoan Leishmania chagasi. Infect. Immun. 62:3262-3269. 363. Windle, J.J., Wiersema, A.K., Clark, J.R., and Feeney, R.E. 1963. Biochemistry 2:1341-1346. 364. Wu, H.F., Monroe, D.M., and Church, F.C. 1995. Characterization of the glycosaminoglycan binding region of lactoferrin. Arch. Biochem. Biophys. 317:85-92. 365. Yamauchi, K., Tomita, M., Giehl, T.J., and Ellison, R.T. 1993. Antibacterial activity of lactoferrin and a pepsin-derived lactoferrin peptide fragment. Infect. Immun. 61:719-728. 366. Yamauchi, K., Wakabayashi, H., Hashimoto, S., Teraguchi, S., Hayasawa, H., and Tomita, M. 1998. Effects of orally administered bovine lactoferrin on the immune system of healthy volunteers. Adv. Exp. Med. Biol. 443:261-265. 367. Yang, H., Kooi, C.D., and Sokol, P.A. 1993. Ability of Pseudomonas pseudomallei malleobactin to acquire transferrin-bound, lactoferrin-bound, and cell-derived iron. Infect. Immun. 61:656-662. 368. Yi, M., Kaneko, S., Yu, D.Y., and Murakami, S. 1997. Hepatitis C virus envelope proteins bind lactoferrin. J. Virol. 71:5997-6002. 369. Yoo, Y.C., Watanabe, S., Watanabe, R., Hata, K., Shimazaki, K., and Azuma, I. 1997. Bovine lactoferrin and lactoferricin, a peptide derived from bovine lactoferrin, inhibit tumor metastasis in mice. Jpn. J. Cancer Res. 88:184-190.
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370. Yoshida, S. 1989. Preparation of lactoferrin by hydrophobic interaction chromatography from milk acid whey. J. Dairy Sci. 72:1446-1450. 371. Yoshida, S., and Ye-Xiuyun. 1991. Isolation of lactoperoxidase and lactoferrins from bovine milk acid whey by carboxymethyl cation exchange chromatography. J. Dairy Sci. 74:1439-1444. 372. Zagulski, T., Lipinski, P., Zagulska, A., Broniek, S., and Jarzabek, Z. 1989. Lactoferrin can protect mice against a lethal dose of Escherichia coli in experimental infection in vivo. Br. J. Exp. Pathol. 70:697-704. 373. Zhao, X.Y., and Hutchens, T.W. 1994. Proposed mechanisms for the involvement of lactoferrin in the hydrolysis of nucleic acids. Adv. Exp. Med. Biol. 357: 271-278. 374. Ziere, G.J., van Dijk, M.C., Bijsterbosch, M.K., and van Berkel, T.J. 1992. Lactoferrin uptake by the rat liver. Characterization of the recognition site and effect of selective modification of arginine residues. J. Biol. Chem. 267:11229-11235. 375. Zimecki, M., Mazurier, J., Machnicki, M., Wieczorek, Z., Montreuil, J., and Spik.G. 1991. Immunostimulatory activity of lactotransferrin and maturation of CD4- and CD8- murine thymocytes. Immunol. Lett. 30:119-124. 376. Zimecki, M., and Machnicki, M. 1994. Lactoferrin inhibits the effector phase of the delayed type hypersensitivity to sheep erythrocytes and inflammatory reactions to M. bovis (BCG). Arch. Immunol. Ther. Exp. (Warsz). 42:171-177. 377. Zimecki, M., Miedzybrodzki, R., and Szymaniec, S. 1998a. Oral treatment of rats with bovine lactoferrin inhibits carrageenan-induced inflammation; correlation with decreased cytokine production. Arch. Immunol. Ther. Exp. (Warsz) 46:361-365. 378. Zimecki, M., Wlaszczyk, A., Cheneau, P., Brunel, A.S., Mazurier, J., Spik, G., and Kubler, A. 1998b. Immunoregulatory effects of a nutritional preparation containing bovine lactoferrin taken orally by healthy individuals. Arch. Immunol. Ther. Exp. (Warsz) 46:231-240. 379. Zimecki, M., Wlaszczyk, A., Zagulski, T., and Kubler, A. 1998c. Lactoferrin lowers serum interleukin 6 and tumor necrosis factor alpha levels in mice subjected to surgery. Arch. Immunol. Ther. Exp. (Warsz) 46:97-104.
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I. INTRODUCTION Lactoperoxidase (LP) is a hemoprotein present in milk, tears, and saliva (Tenovuo & Pruitt, 1984) ). LP constitutes one of the nonimmunoglobulin defense factors in the mucosal secretions (Mandel & Ellison, 1985). In 1881, Arnold demonstrated the peroxidase activity in bovine milk. Later in 1943, Theorell and Åkeson, isolated the protein responsible for this enzyme activity, by precipitation methods, and termed ‘lactoperoxidase’. The purification of LP has been considerably refined in the later years by several groups. Subsequent studies have analyzed the amino terminus, along with amino acid and carbohydrate composition (Rombauts et al., 1967; Carlstrom, 1969; Sievers, 1981; Paul & Ohlsson, 1985). These studies further suggested that LP could exist in multiple forms, probably reflecting heterogeneity in glycosylation. LP contains at least two domains differing in thermostability (Pfeil & Ohlsson, 1986). In addition, a peroxidase with similar biochemical and immunological properties, which could originate from the same gene as LP, has been found in human saliva (Mansson-Rahematulla, 1988). The gene sequences encoding several peroxidases including LP has been published (Dull et al., 1990). The involvement of LP in the inhibition of microbial growth (stasis) was first suggested by Hanssen (1924) and was ultimately demonstrated by Wright and Trammer (1958). Involvement of hydrogen peroxide (Jago & Morrison, 1968) and thiocyanate (Reiter et al., 1963) in the inhibitory phenomenon was observed. Earlier, this stasis effect was considered as a limitation in the manufacture of cultured dairy products from normal cow milk, which contains large amounts of LP and thiocyanate. Later, it was suggested that the presence of LP in the mammary, salivary, lacrimal and harderian glands may constitute a naturally occurring defense mechanism in the body to control microbial proliferation (Klebanoff & Luebke, 1965; Slowey et al., 1968). Hydrogen peroxide is cidal to a variety of life forms inspite of their highly developed defense mechanisms against this oxidizing agent (Chance et al., 1979). Thus, free hydrogen peroxide may pose a threat to both human and microbial cells. Hydrogen per-
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oxide is a substrate for LP in oxidizing thiocyanate (SCN-) to hypothiocyanate (OSCN) (Thomas, 1985). Several studies have suggested that the peroxidation reaction serves at least two important functions in the mucosal secretions: 1) the products of the reaction lead to antimicrobial activity (Pruitt & Reiter, 1985); and 2) the reaction prevents the accumulation of hydrogen peroxide excreted by many microorganisms (Carlsson et al., 1983) and host cells (Pruitt et al., 1983). Hydrogen peroxide is highly toxic to mammalian cells and is consumed rapidly by the peroxidase reaction into nontoxic byproducts (Hanström, 1983). The LP system also inhibits hexokinase (Adamson & Pruitt, 1981) and glyceraldehye-3-phosphate dehydrogenase (Carlsson et al., 1983). The enzyme inhibitory activity could contribute to the antimicrobial function of the LP system. The LP system has been suggested to protect the gut of the calf from enteric pathogens (Reiter et al., 1980) and a possible role for LP in the defense of the mammary gland has been postulated (Reiter & Bramley, 1975). LP has been used to preserve milk without refrigeration (Bjorck et al., 1979). The LP system could inhibit bacteria, fungi, parasites and viruses; therefore, it is considered as a broad-spectrum natural antimicrobial for food safety and preservation.
II. OCCURRENCE LP is the most abundant enzyme in bovine milk, constituting about 1% of the whey proteins or 10-30 µg/ml of milk (Reiter, 1985). Feeding practices could influence the LP levels (Kiermeier & Kuhlmann, 1972), and elevated somatic cell counts correlate with increased LP levels in bovine and human milk (Gothefors & Marklund, 1975). The concentration of LP is low in the bovine colostrum and increases rapidly to reach a peak at 4-5 days of postpartum. It declines rapidly afterwards to reach a constant, rather high, plateau during the lactation. Human LP concentration is high in colostrum and declines rapidly within 1 week (Kiermeier & Kuhlmann, 1972; Gothefors & Marklund, 1975). The concentrations of LP and SCN- in the bovine mammary secretions during the early dry period are similar to the milk before drying off. However, the free cysteine levels progressively increase in the secretions beginning 3 to 5 days after the last milking. The secretions, when diluted in steamed milk, show greater stimulation of Streptococcus agalactiae growth as the drying-off period progresses. This effect has been attributed to the increased concentrations of cysteine that counteracts the LP/SCN-/ H2O2 inhibitory system for S. agalactiae. This effect on the LP system has been suggested to increase the susceptibility of bovine udder to S. agalactiae infection during the dry period (Brown & Mickelson, 1979). Milk from infected udders shows higher levels of LP and SCN- than milk from normal udders. Udder irritation could increase bacteriostatic activity of milk (JanotaBassalik et al., 1977). Estrogen could also influence the LP concentration in bovine milk. Thus, the peroxidative activity of milk varies periodically in non-pregnant but not in pregnant cows. The milk of cows in estrus shows increased LP activity and turns normal after ovulation (Kern et al., 1963). LP concentration in cervical mucus significantly drops after ovulation (Linford, 1974). Immunofluorescence and hybridization techniques revealed the localization of LP in the goat lactating mammary gland (Cals et al., 1994). In situ hybridization experiments have demonstrated the presence of LP mRNA within the cytoplasm of alveolar epithelial cells (acini). © 2000 by CRC Press LLC
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FIGURE 1: Isolation of lactoperoxidase on Bio-Rex 70 resin column at 4 °C by ion-exchange chromatography. The column was equilibrated with starting buffer (0.02 M sodium acetate, pH 7.35) at a flow rate of 30 ml/h. The absorbance of fractions was measured at 280 mµ ( thin line) and 412 mµ (line with circles). At the end of the first gradient (dotted line) the green LPO was located on the top of the column and a more gradual gradient with 0.35 M sodium acetate, pH 7.9 (dotted line) completely eluted the enzyme. The fractions with an A412:A280 ratio (thick line) above 0.9 were pooled and concentrated (redrawn from Rombauts et al., 1967).
Pruitt et al. (1990) described an assay to measure peroxidase concentration in biological fluids. Regression equations were used to calculate concentrations of bovine LP, human salivary peroxidase, and human myeloperoxidase. Electron donors: pyrogallol, guaiacol, 2,2’-azinobis (3-ethylbenzylthiazoline-6-sulfonic acid, ABTS), and thiocyanate (SCN-) were used to measure the peroxidase activity. The peroxidation rates of these donors depend upon the concentrations of H2O2, thus, should be carefully controlled for accurate, and reproducible results.
III. MOLECULAR PROPERTIES A. Isolation and Purification Casein precipitation with rennet and adsorption of whey proteins to ion exchangers are basic steps in the isolation and purification of LP (FIGURE 1). Paul and co-workers (1980) described a method that minimizes extreme ionic fluctuations, and avoids over exposure to potassium phosphate. Unpasteurized skim milk is coagulated with rennin (2 mg/L). After cooling with ice, the whey is stirred for 3-h with the ion exchanger CG-50NH4 (20 g/L). The LP-resin complex after two washes with water, three washes with 50 mM sodium acetate, is transferred to a column and allowed to settle in 50 mM sodium acetate buffer under cautious stirring to prevent channeling. LP is eluted with 2 M sodium acetate and transferred to a phenyl-Sepharose column. LP is further eluted with
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decreasing, linear gradient of sodium acetate (2.0-0.5M, pH 7.0). The eluate is concentrated in a Diaflow XM-50 cell with slow stirring, dialyzed against 10 mM sodium phosphate (pH 6.0). The dialysate is fractionated by chromatography on CM-52 with a sodium phosphate gradient (10-130 mM, pH 6.0). The final purification and separation of LP subfractions is performed on DEAE-Sephadex. Borate (10 mM, pH 9.0 and 8.0) resolves LP into a number of fractions. Human LP with stability and immunoreactive properties similar to that of bovine milk LP has been partially purified from human colostrum by hydrophobic interaction chromatography (Langbakk & Flatmark, 1984). A 10-fold purification with an apparent recovery of about 45% was obtained by using Phenyl-Sepharose C1-4B. A procedure for isolation and purification of LP from cow milk was described by Denisova et al. (1986). This procedure involves isolation of casein from milk, sorption of LP on CM-Sephadex, concentration of the eluate using ultrafiltration, salting out with ammonium sulfate and a final isoelectric focusing in borate-polyol system. Highly purified, active preparation of LP was obtained within a relatively short period by this procedure. Ferrari and co-workers (1995) developed an improved purification method for LP using preparative chromatography and electrophoresis methods combined with analytical electrophoresis techniques and image processing. Electron paramagnetic resonance (EPR) analysis has been used to evaluate LP homogeneity against lactoferrin and minor LP components to define the final steps of purification. Two samples of LP (from farm and commercial milk) were purified and characterized by EPR spectroscopy to clarify the Fe(III)-heme high-spin nature of the native LP. These data indicated the presence of an iron(III)-heme high-spin catalytic site in the native enzyme. In contrast, LP from commercial milk, a low-spin iron(III)-heme species, was observed due to nitrite impurities. The LP/SCN- activity in phosphate and acetate buffer was optimal at pH 5.5. A fractionation scheme for isolation LP, lactoferrin, and IgG, based on cation exchangers was developed (Hahn et al., 1998). Four different cation-exchange media (SHyperD-F, S-Sepharose FF, Fractogel EMD SO3- 650 (S) and Macro-Prep High S Support) were compared for dynamic binding capacity to IgG and different elution behaviors with sequential step gradients of NaCl buffers. Peak fractions were analyzed by sizeexclusion chromatography and sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE). LP activity was monitored by the oxidation of O-phenylenediamine. Fractogel EMD had the highest binding capacity for IgG (3.7-mg/ml gel at a linear flowrate of 100 cm/h), however, the resolution was low compared to the other three media. SHyper D and S-Sepharose FF showed lower capacities (3.3 and 3.2-mg/ml gel, respectively) but exhibited better protein resolution. These effects could be partially explained by the k’ versus salt concentration plots. The binding capacity of Macro-Prep S was considerably lower compared to that of the other resins. S-Sepharose FF and S-Hyper D combine relatively high dynamic capacity for IgG and provided good resolution. Compared to studies with standard proteins, such as 100-mg/ml bovine serum albumin for S-Hyper D, their binding capacities were very low. Even after removal of low-molecular-mass compounds, the capacity could not be improved significantly. The running conditions (low pH) were responsible for the low protein binding capacity, since low-molecular-mass compounds in the feed do not compete with the adsorption of whey protein. The dynamic capacity did not decrease to a large extent within the range of flow-rates (100-600 cm/h)
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investigated. The dynamic capacity of HyperD and Fractogel was at least five times higher when pure bovine IgG was used for determination. In conclusion, S-Sepharose FF, SHyper D-F and Fractogel EMD SO3- 650 (S) are considered as successful candidates for the large-scale purification of bovine whey proteins. B. Chemistry and structure Early ORD studies with LP in the far ultraviolet region indicated a 17% alphahelical structure (Maguire & Dunford, 1971). Later evaluation of optical and CD spectra revealed 65% beta-structure, 23% alpha-helix, and 12% unordered structure for LP (Sievers, 1980). Reducing SDS-PAGE with 1% SDS/mercaptoethanol showed a single component, indicating only one peptide chain. Dansylation revealed only one N-terminal amino acid, leucin. LP contains 8 disulfide bonds that contribute to the rigidity of the molecule. The single peptide chain of bovine LP contains 612 amino acid residues, including 15 half-cystines and 4 or 5 potential N-glycosylation sites. The corresponding peptide segments of human myeloperoxidase, eosinophil peroxidase and thyroperoxidase display 55%, 54% and 45% identity with bovine LP, respectively, with 14 out of the 15 half-cysteines present in each of the four enzymes being located in identical positions (Cals et al., 1991). The occurrence of an odd number of half-cysteines in bovine LP supports the finding of a heme thiol released from this enzyme by a reducing agent, suggesting that the heme is bound to the peptide chain via a disulfide linkage. The amino acid composition of LP is compared with salivary peroxidase and myeloperoxidase in TABLE 1. Peptide sequences obtained from cyanogen bromide fragments of bovine LP were used to design oligonucleotide probes for cDNA library screening constructed from bovine mammary tissue (Dull et al., 1990). Three overlapping clones were obtained, the longest of which (T3) contained a reading frame of 712 amino acid residues. The encoded amino acid sequence was homologous to those reported for myelo-, thyro-, and eosinophil peroxidases. Two possible amino termini of the mature enzyme were identified, and the predicted mature protein matched previous molecular weight estimates of 78,500. Of eight bovine tissues tested, transcription of T3 sequences were detected in mammary tissue only. Using the bovine LP cDNA as a probe, a single hybridizing clone was found in a human mammary gland cDNA library. This clone encoded the carboxyterminal 324 residues of a peroxidase distinct from the other three known human peroxidases, and was closely related to bovine LP. Ueda and co-workers (1997) reported the molecular cloning of human LP chromosomal gene and determined its gene organization. The human LP gene is arranged with the myeloperoxidase gene in a tail-to-tail manner. Similar to the human myeloperoxidase and eosinophil peroxidase genes, the human LP gene was split by 11 introns and spans 28 kb. Unlike most introns in mammalian gene, the 5’ splice donor sequence of intron 11 starts with GC instead of GT. When the minigene comprised of exon 11, intron 11 and exon 12 of the human LP gene was introduced into COS cells, the correct splicing of the intron was found, suggesting the intron 11 of the human LP gene was functional. The coding sequence of human LP consists of 2136 bp, and codes for a protein of 712 amino acids. The amino acid sequence of human LP showed 51% homology with human myeloperoxidase and eosinophil peroxidase, suggesting that these peroxidase genes have evolved from a common ancestral gene. On the other hand, the nucleotide sequences of the 5’ promoter regions of these peroxidase genes exhibit no similarity, which agrees with their tissue-specific expression. © 2000 by CRC Press LLC
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TABLE 1: Comparison of aminoacid composition in lactoperoxidase, salivary peroxidase and myeloperoxidases Amino acid Aspartic acid Threonine Serine Glutamic acid Proline Glycine Alanine Cysteine Valine Methionine Isoleucine Leucine Tyrosine Phenylalanine Lysine Histidine Arginine Tryptophan
Bovine LP 127 50 60 107 80 77 69 15 40 16 32 113 27 52 55 23 61 ND
Human SP 118 49 77 105 97 77 74 16 38 5 31 117 22 50 50 18 57 ND
Human MP 132 56 54 136 84 76 72 24 48 24 32 60 24 48 24 12 96 12
(Adapted from Cals et al., 1991; Matheson et al., 1981; Mansson-Rahemtulla et al., 1988)
C. Stability During pasteurization, whole milk loses about three-quarters of LP activity, whereas partially purified LP is stable for 15 min at this temperature (Wutrich et al., 1964). Kinetic studies of the rate of formation of Compound-I indicated that LP is stable when stored at neutral pH 7.0 but deactivates by storage at acidic pH 3.0 (Maguire et al., 1971). The deamidization of LP by glycine at pH 10.3 for 48 hr at room temperature seemed not to inactivate LP. No heme was released by acid butanone after digestion of LP with pepsin followed by trypsin (Morell, 1953) or chymotrypsin (Sievers, 1979). Also trypsin and thermolysin did not inactivate native LP, while chymotrypsin caused a moderate effect. Pronase rapidly digests native LP to fragments from which heme could be extracted (Sievers, 1979). LP is not inactivated by the gastric juice (pH 5.0), whereas pepsin at pH 2.5 inactivated LP (Gothefors & Marklund, 1975). The prosthetic group of milk LP has been isolated from a pronase hydrolysate of the enzyme and identified as protoheme IX (Sievers, 1979). Partial degradation of the heme occurs during the proteolysis, possibly because of coupled oxidation in the presence of glycine and oxygen. The heme seems to be buried in the protein molecule in a crevice that allowed ligands to bind to the iron on one side only. Pfeil and Ohlsson (1986) studied the thermal unfolding of LP by differential scanning calorimetry and optical methods. The protein demonstrated at least two domains differing in thermostability. The prosthetic group belonged to the domain of lower thermostability. Thermodynamic parameters of protein unfolding were found similar to the globular proteins. Marcozzi and co-workers (1998) investigated the activity and the stability of bovine LP in the presence of different surfactants. The cationic benzalkonium chloride was effective in preserving the enzymatic activity for over 10 days, while the native LP
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completely lost its activity within 3-4 days. In the presence of benzalkonium chloride, LP could preserve its secondary structure for a long time. This condition creates an enhanced hydrophobic environment for LP, as indicated in fluorescence studies. Moreover, this surfactant at a concentration of 0.01% (0.3 mM) increased the LP activity in the first 2-h of incubation at 37ºC. Both hydrophobic and electrostatic interactions of the cationic surfactant seem to be responsible for the enzyme activation and stabilization. D. Heterogeneity Two different molecular forms of LP were reported, probably representing a monomer and an aggregate (Tenovuo, 1981). The isoelectric point of LP (pI, 8.1) did not change during aggregation. The presence of substrate (SCN-) caused some disaggregation. Purified milk LP showed a similar chromatographic pattern to salivary LP. Two distinct LP forms, a non-heme and an enzymatically active LP were isolated from bovine milk by Dumontet and Rousset (1983). Both forms of LP demonstrated similar molecular weight of 85-kDa in the denatured (SDS-PAGE) and native form (velocity sedimentation on sucrose gradient). However, the non-heme form was devoid of light absorption properties in the Soret region and of enzyme activity. Both forms showed similar carbohydrate content and peptide maps after limited proteolysis by subtilisin or trypsin. The two forms showed immunological relatedness in immunodiffusion and radioimmuno assays. The non-heme LP was readily detected in milks from cow, goat, sheep, and human species. In bovine milk, LP and non-heme LP were found in comparable amounts. Antibodies raised against bovine LP moderately cross-react with human salivary peroxidase. In double-immunodiffusion experiments, the two enzymes show partial identity, and in competitive radioimmunoassay and enzyme-linked immunosorbent assay, Western blot analysis differentiate salivary peroxidase from human and rat saliva samples and the purified enzyme in its non-reduced, reduced, and de-glycosylated forms. The major activity of these antibodies was directed against the protein core of the antigen. Immunodetection of the peptide fragments of bovine LP and human salivary peroxidase revealed structural differences in the two enzymes (Masson-Rahematullah et al., 1990). E. Molecular interactions LP interacts with other components of milk and saliva, and this interaction could be significant in vivo. LP binds to secretory IgA, IgM, myeloma IgA1, and myeloma IgA2 (Tenovuo et al., 1982). The interactions between LP and the immunoglobulins are nonspecific. The LP-Ig complex was more stable than the free enzyme. However, LP does not bind to IgG or lactoferrin. The interaction of LP with lysozyme and ribonuclease from cow milk has also been reported (Hulea et al., 1989). LP is slightly activated when complexed to lysozyme, while IgA and IgM were inhibitory. On the other hand, IgG and ribonuclease had no effect on the enzyme activity although the latter did form a complex with the LP. The interaction between LP and lysozyme appears to be lectin-type since the alteration of LP sugar moiety by periodate oxidation, prevented the formation of the LPlysozyme complex. The interaction of bovine LP with several inorganic species including SCN-, I-, Br-, Cl-, F-, NO2-, N3-, CN- was reported (Ferrari et al., 1997). Based on the ability of LP to form 1:1 complexes with the above ligands and the dissociation constant values (Kd) of
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the adducts, three groups were observed: 1) SCN-, I-, Br-, and Cl- (Kd increases along the series); 2) F- (which shows a singular behavior); 3) NO2-, N3-, and CN- (that bind at the iron site). Kd values for the LP/SCN- adduct were altered in the presence of other inorganic species; a strong competition between the substrate and all other anions (with the exception of F-) was observed. Binding studies on the natural substrates SCN- and I- indicated protonation of a common site in proximity of the iron (possibly distal histidine). Computer-assisted docking simulations suggested the ability of all ligands to penetrate the heme pocket.
IV. ENZYME ACTIVITY Peroxidases belong to a group of enzymes that catalyze the oxidation of numerous organic and inorganic substrates by H2O2. Most peroxidases, including LP contain ferriprotoporphyrin IX as a prosthetic group. A characteristic feature of hemoprotein peroxidases is their ability to exist in various oxidation states. There are five known enzyme intermediates. In increasing order of their oxidative equivalents, these are ferrous enzyme, ferric or native enzyme, Compound-II, Compound-I, and Compound-III. They are readily distinguished from each other by their absorbance in the Soret region (380-450 nm) and visible range (450-650 nm). In the course of Compound III and Compound-II conversion back to the native peroxidase, oxygen-derived free radicals such as O2-, HO2., and .OH are generated. Simultaneously the enzyme is irreversibly damaged. In the presence of an exogenous electron donor, such as I-, the interconversion between the various oxidation states of the peroxidase is markedly affected. Compound-II and/or Compound-III formation is inhibited, depending on the H2O2. In addition, the enzyme is largely protected from irreversible inactivation. These effects of I- are readily explained by a) the two-electron oxidation of I- to Iox by Compound-I, which bypasses Compound-II as an intermediate and b) the rapid oxidation of H2O2 to O2 by the oxidized species of I- which prevents the generation of oxygen derived free radicals (Kohler & Jenzer, 1989). Piatt and O’Brien (1979) reported the evidence for singlet oxygen formation for the LP/H2O2/Br- system by monitoring 2,3-diphenylfuran and diphenylisobenzofuran oxidation, O2 evolution, and chemiluminescence. This mechanism provided an explanation for the cytotoxic and microbicidal activity of peroxidases and polymorphonuclear leukocytes. Evidence for singlet oxygen formation included: • Chemiluminescence accompanying the enzymatic reaction was doubled in a deuterated buffer and inhibited by singlet oxygen traps. • Singlet oxygen traps, diphenylfuran and diphenylisobenzofuran, were oxidized to their known singlet oxygen oxidation products in the presence of LP/H2O2/Br-. • Rate of oxidation of diphenylfuran and diphenylisobenzofuran was inhibited when monitored in the presence of known singlet oxygen traps or quenchers. • Singlet oxygen traps inhibited oxygen evolution from the enzymatic reaction but not by singlet oxygen quenchers. • Traps or quenchers which were effective inhibitors in the experiments above did not inhibit peroxidase activity, were not competitive peroxidase substrates and did not react with the hypobromite intermediate since they did not inhibit hydrogen peroxide consumption by the enzyme.
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Pruitt and co-workers (1982) examined the LP-catalyzed oxidation of SCN- by two different polarographic techniques: direct current polarography and linear sweep voltametry. The main oxidation product at pH 6.5, with a half-wave potential (Efi) of -0.39 to -0.44 V, was identified as OSCN- ion. All three components of the LP system (i.e. LP/SCN-/ H2O2) were required to produce OSCN-. Addition of excess H2O2 or H2O2/LP to an OSCN-/SCN- mixture generated a new peak associated with a simultaneous decrease of OSCN- concentration. This indicates a possible reaction between H2O2 or H2O2/LP and OSCN-. This new peak possibly represents higher oxy acids of SCN(O2SCN-, O3SCN-), formed in the oxidation of OSCN- by H2O2 or by H2O2/LP. This reaction might explain why, in solutions that already contain OSCN- (e.g., in saliva), the addition of H2O2 results in the formation of highly reactive, short-lived antimicrobial products in addition to OSCN-. The heme environmental structures of LP have been studied by the use of hyperfine-shifted proton NMR and optical absorption spectra (Shiro & Morishima, 1986). The NMR spectra of the enzyme in native and cyanide forms in water indicated that the fifth ligand of the heme iron is the histidyl imidazole with an anionic character and that the sixth coordination site is possibly vacant. These structural characteristics are quite similar to those of horseradish peroxidase (HRPO), suggesting that these may be prerequisite to peroxidase activity. LP-catalyzed H2O2 metabolism proceeds through one of three different pathways, depending on the nature and the concentration of the second substrate as an electron donor and/or on pH conditions (Jenzer et al., 1986). In the LP/H2O2, at low H2O2 levels and/or alkaline conditions the peroxidative cycle involves ferric LP/Compound-I/ Compound-II/ferric LP conversion, whereas high H2O2 levels and/or acidic conditions favor the ferric LP/Compound-I/Compound-II/Compound-III/ferrous LP/ferric LP pathway. The Compound-III/ferroperoxidase states are associated with irreversible enzyme inactivation by cleavage of the heme moiety and liberation of iron. It is likely that either singlet oxygen or superoxide and hydroxyl radicals are involved in the attack on heme iron, because inactivation correlates with oxygen production and can be decreased to a certain degree by scavengers such as ethanol, 1-propanol, 2-propanol, or mannitol. In the LP/ H2O2/I- system, the enzyme may also be inactivated by iodide generated in the course of enzymatic I- oxidation (i.e. during ferric LP/Compound-I/ferric LP cycles). The LP-catalyzed oxidation of glutathione (GSH) and SCN- was studied (Lovaas, 1992). One or two moles of GSH were oxidized per mole of H2O2, depending on the reaction conditions. Omission of SCN- prevented the oxidation of GSH. The oxidation of GSH required only catalytic amounts of SCN-, which was therefore recycled. Iodide (I-) could replace SCN-, while chloride or bromide was ineffective. The apparent Michaelis constant for SCN- was 17 µM. Oxidation of SCN- generated two reactive intermediates, one stable and one unstable. The stable intermediate (-OSC.) decayed by a second-order reaction. The decay of the unstable radical was very fast. These data elucidate the short- and long-term antibacterial effects of LP/halide/ H2O2; point to possible deleterious effects due to glutathione depletion; and support observations on lipid peroxidation/ halogenation in biological membranes, liposomes, and unsaturated fatty acids. Products formed from the LP catalyzed oxidation of SCN- with H2O2 was studied by 13C-NMR at pH 6.0 and 7.0 (Pollock & Goff, 1992). Ultimate formation of OSCN-
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as the major product correlates well with the known optical studies. The oxidation rate of SCN- appears to be greater at pH < or = 6.0. At H2O2/SCN- ratios of < or = 0.5, OSCNwas not formed immediately, but an unidentified intermediate was produced. At H2O2/SCN- ratios of > 0.5, SCN- appears to be directly oxidized to OSCN-. Once formed, OSCN- slowly degrades over a period of days to CO2, HCO3-, and HCN. An additional product also appears after formation of OSCN-. On the basis of carbon-13 chemical shift information this new species was suggested to result from rearrangement of OSCN- to yield the thiooxime isomer, SCNO- or SCNOH. It should be noted that the final product of LP reaction depends on the method of H2O2 generation and relative proportions of the substrates (Dionysius et al., 1992).
V. ANTIMICROBIAL ACTIVITY Peroxidase enzymes catalyze the oxidation of electron donors by peroxide to generate highly reactive products with a wide range of antimicrobial properties. The actual structures of these products and the chemistry of their reactions depend upon the specific peroxidase-electron donor pair. The SCN- ion is the most significant electron donor in vivo, which is a normal constituent of bovine milk and is derived from the diet. The major end product of the LP/SCN- at neutral pH is the OSCN- anion, which is in equilibrium with hypothiocyannous acid (HOSCN, pK 5.3) (Thomas, 1981). There are other products of the LPS/SCN- that are generated in small amounts and are relatively unstable at neutral pH compared to SCN- (Aune & Thomas, 1977; Bjorck & Clasesson, 1980; Pruitt & Tenovuo, 1982). A. Mechanism(s) of action The antibacterial activity of the LP/SCN-/ H2O2 system has been suggested due to the OSCN- anion. Relatively pure solutions of OSCN- could be prepared using an immobilized enzyme. To support the above hypothesis pure OSCN- preparations were directly tested for antimicrobial effects on Escherichia coli and Streptococcus lactis (Marshal & Reiter, 1980). E. coli was killed in the presence of OSCN- anion whereas the effect on Streptococcus lactis was only bacteriostatic. These studies supported the similarities of LP/SCN-/ H2O2 and OSCN- systems. The cellular targets for OSCN- and HOSCN interaction are sulfhydryl groups (Aune & Thomas, 1978) and reduced nicotinamide nucleotides (Oram & Reiter, 1966). The sulfhydryl groups could be the cysteine residues of specific proteins or reduced GSH. Sulfhydryl groups are oxidized to disulfides (-S-S-), sulfenyl thiocyanates (-S-SCN-), and sulfinic acids (-S-OH). Disulfides, sulfenyl thiocyanates, and sulfinic acids are readily converted back to sulfhydryls by an excess of reducing agents such as cysteine, mercaptoethanol, dithiothreitol, sodium hydrosulfite and GSH. The nucleotides NADH and NADPH are oxidized to NAD+ and NADP+, and this reaction is also reversible. LP is effective at concentrations as low as 0.5 µg/L (about 6.5 x 10 –12 M, assuming a Mr of 77 kDa). LP catalyzes the oxidation of SCN- by H2O2 into OSCN-, a reaction that could protect bacterial and mammalian cells from killing by H2O2. Carlsson and co-workers (1984) demonstrated, however, that LP in the presence of SCN- could potentiate the bactericidal and cytotoxic effects of H2O2hydrogen under specific conditions, such as when
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H2O2 is present in the reaction mixtures in excess of SCN-. The toxic agent was also formed in the absence of LP in a reaction between OSCN- and H2O2. Sulfate, sulfite, cyanate, carbonate, and ammonia, generated during the OSCN- oxidation by H2O2 were not bactericidal and did not potentiate the bactericidal effect of H2O2. The authors suggested that cyanosulfurous acid, the only other postulated product of the chemical oxidation of OSCN- by H2O2, as the possible cidal agent. Adsorption of LP to microbial cell surface seems necessary to elicit antimicrobial effects (Tenovuo & Knuuttila, 1977). There have been conflicting reports regarding the binding of LP to bacterial cell surfaces. Effects of bacterial cell-bound LP on acid production by suspensions of Streptococcus mutans in the presence of H2O2 and SCN- was reported (Pruitt et al., 1979). Addition of H2O2 and SCN- to bacterial cells treated with LP (0.1 mg/ml and thoroughly washed) caused marked reduction in acid production by S.mutans. After a 3-h incubation in saline, however, the LP-treated bacteria produced acid in the presence of H2O2 and SCN-. The authors concluded that LP is initially bound to the bacterial cell surface in an enzymatically active form at a concentration sufficient to inhibit acid production. The LP seems to slowly degrade or desorb as the bacteria stand in saline suspension. Mickelson (1979) reported that low amounts of LP adsorb to the cell surface of S. agalactiae and are not removed by washing. A diffusible antibacterial product of LP/H2O2/SCN-reaction was not detected. Incubation of S. agalactiae cells with LP/H2O2 and 14C-labeled sodium SCN resulted in the incorporation of SCN into the bacterial protein. Most of the LP-catalyzed, incorporated SCN was released from the bacterial protein with dithiothreitol. Cells that had their membrane permeability changed by treatment with Cetab or 80% ethanol incorporated more SCN than did untreated cells (about 1 mol of SCN for each mol of sulfhydryl group present in the reaction mixture). Alteration of membrane permeability caused protein sulfhydryls, normally protected by the cytoplasmic membrane, to become exposed to oxidation. It was suggested that LP/H2O2-catalyzed the incorporation of SCN into the proteins of S. agalactiae by a mechanism similar to that reported for bovine serum albumin. It was speculated that the removal of reactive protein sulfhydryls from a functional role in membrane transport and in glycolysis has a possible role in eliciting antibacterial effect for S. agalactiae. LP is enzymatically effective even when fewer than 100 molecules are adsorbed per cell of Streptococcus mutans (Pruitt et al., 1979). B. Antimicrobial target sites Cytoplasmic membrane and/or cytoplasm are suggested to be major targets for antimicrobial products of the LP system. The cell wall and outer membrane may partially limit accessibility but do not totally exclude the products of the LP/SCN- from the cell interior. The cell wall of E. coli may also be altered by exposure of cells to the LP/SCN(Reiter, 1978). Marshall and Reiter (1980) reported the ability of OSCN- to alter bacterial cytoplasmic membranes. Treatment of E. coli suspensions with OSCN- caused extensive leakage of [14C] amino acids and 42K in 10 min. Damage to the inner membrane of E. coli was also suggested by the increase in hydrogen ion permeability of cells treated with the LP/SCN- (Law & John, 1981). The cell walls of gram-positive bacteria are less susceptible to damage by the products LP system than of gram-negative bacteria. © 2000 by CRC Press LLC
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The cytoplasmic membrane of gram-positive bacteria is also altered by the LP system. Treatment with the LP system or OSCN- could inhibit amino acid transport in Lactobacillus acidophilous (Clem & Klebanoff, 1966; Slowey et al., 1968) and S. aureus (Hamon & Klebanoff, 1973), and glucose and oxygen uptake in numerous species. Mickelson (1977) found that the LP/SCN- inhibits glucose transport system of S. agalactiae by modification of essential membrane sulfhydryl groups. Later studies indicated that the LP system incorporated S14CN- into bacterial protein which could be released by treatment with reducing agents (Mickelson, 1979). Antimicrobial products of LP system could inhibit several glycolytic enzymes including hexokinase, aldolase, 6-phosphogluconate dehydrogenase and glucose-6-phosphate dehydrogenase activities in Streptococcus cremoris (Oram & Reiter, 1966). Similar enzyme inhibition was also observed with S. mutans. Thus, LP-treated cells show marked reduction in pyruvate kinase, hexokinase, and aldolase activities. However, the levels of enolase phophoglycerate kinase and phosphoglycerate mutase were slightly affected (Hoogendoorn, 1974). Glyceraldehyde-3-phosphate dehydrogenase activity of S. pyogenes is inhibited by LP/H2O2 mixtures in the absence of SCN- (Mickelson, 1966). Later studies also showed that OSCN- could directly oxidize glyceraldehyde-3-phosphate-dehydrogenase (Carlsson et al., 1983). Treatment of cell extracts of this enzyme (NAD linked) from S. mitis, S. sanguis, S, mutans and S. salivarius with OSCN- solutions resulted in complete inhibition of enzyme activity. C. Regulating factors Concentration of LP is not a limiting factor for antibacterial activity in bovine milk or in human saliva. However, the SCN- concentration is a limiting factor in milk and sometimes in saliva, but usually it is the availability of H2O2 that determines the magnitude of antibacterial activity of peroxidase systems (Pruitt et al., 1982). Susceptibility of microorganisms to the antimicrobial activity of LP is dependent on the state of their metabolic growth. In general, resting cells or cells in the stationary growth phase are more susceptible to killing or inhibition than are metabolically active or growing cells. Bacteria grown anaerobically are more susceptible to LP than are those grown aerobically (Carlsson et al., 1983). Also the increased permeability of the cell envelope is associated with increased susceptibility to LP-mediated antibacterial effects (Purdy et al., 1983). Under aerobic conditions, LP and SCN- could protect E. coli and oral streptococci from the bactericidal effect of H2O2 (Adamson & Carlsson, 1982). LP in the absence of SCN- was protective but potentiated H2O2 toxicity for certain other bacterial species under similar conditions. The products of reaction between H2O2 and SCN- in the presence of LP were not bactericidal except for E. coli. Inhibition of bacterial metabolism by the LP/SCN-/H2O2 system was studied with serotypes A through G of S. mutans (Thomas et al., 1983). When the washed, stationary-phase cells were incubated aerobically with LP/SCN- and glucose, > 90% inhibition of sugar utilization and lactate production was obtained with strains that released large amounts of H2O2; 20 to 50% inhibition was obtained with strains that released about half as much H2O2; and no inhibition was obtained with strains that released only small
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amounts of H2O2. Inhibition was most effective at pH 5.0, whereas release of H2O2 and accumulation of the inhibitor (OSCN- ion) were highest at pH 8.0. With H2O2-releasing cells from early stationary phase, preincubation with glucose abolished inhibition, though it did not influence H2O2 release. Cells harvested 24 h later were depleted of sulfhydryl compounds. Inhibition of these cells was abolished by preincubation with glucose and certain sulfhydryl or disulfide compounds (reduced or oxidized GSH, cysteine or cystine). This preincubation increased cell sulfhydryl content but had no effect on H2O2 release. All strains were inhibited when incubated with LP/SCN- and added (exogenous) H2O2. Smaller amounts of H2O2 were required to inhibit at pH 5.0, and larger amounts were required to inhibit cells preincubated with glucose alone or in combination with sulfhydryl or disulfide compounds. The results indicate that pH, amount of H2O2, cell sulfhydryl content, and stored-carbohydrate content determine susceptibility to inhibition. Cystine reduction in S. agalactiae, resulting in sulfhydryl formation, may account for antagonism of the antibacterial effect of LP/SCN-/H2O2 system when cystine is present in excess (Mickelson & Anderson, 1984). The reduction of cystine seems to occur by a coupling reaction between GSH reductase and GSH-disulfide transhydrogenase activity, both of which were found in the supernatant fraction from cell homogenates. NADPH-specific GSH reductase activity was found in the pellet and supernate fractions from cell homogenates. Two sulfhydryls were formed for each mole of NADPH used during cystine reduction. Excess amounts of I- (10 mM) and H2O2 (0.1-10 mM) could cause rapid, irreversible inactivation of LP without forming Compound III (Huwiler et al., 1986). In contrast, in the absence of I- Compound III was formed and inactivation proceeded in a slow fashion. Increasing the LP concentration accelerated the rate of inactivation. Irreversible inactivation of LP involved cleavage of the prosthetic group and liberation of heme iron. The rate of enzyme destruction was correlated with the production of molecular oxygen (O2), which originated from the oxidation of excess H2O2. Since H2O2 and O2 per se do not affect the heme moiety of the peroxidase, it was suggested that the damaging species may be a primary intermediate of the H2O2 oxidation, such as oxygen in its excited singlet state, superoxide radicals, or consequently formed hydroxyl radicals. Jenzer and Kohler (1986) have investigated irreversible inactivation of LP in the presence of excess H2O2. Serial overlay absorption spectra of the Soret region indicated that the rate and total amount of enzyme inactivation depend on the proton concentration. Perhydroxyl or superoxide radicals could not be established as the inactivating species in this mechanism; however, these radicals could influence the rate of reconversion of the intermediate LP-compound III back to the resting ferric form. The irreversible inactivation of bovine LP by thiocarbamide goitrogens was reported, and the kinetics were consistent with a mechanism-based (suicide) mode (Doerge, 1986). Sulfide ion-inactivated, 2-mercaptobenzimidazole-inactivated, and 1methyl-2-mercaptoimidazole-inactivated LP demonstrated different visible spectra, suggesting the formation of various products. These data support a mechanism in which reactive intermediates are formed by S-oxygenation reactions catalyzed by LP Compound II. It was proposed that the reaction of electron-deficient intermediates with the heme prosthetic group was responsible for the observed spectral changes and inactivation by thiocarbamides.
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The oxidation of SCN- by H2O2 in the presence of LP does not take place at pH greater than 8.0. Since SCN- does not bind to LP above this pH, the binding of SCN- to LP is considered to be prerequisite for the oxidation of SCN-. Maximum inhibition of oxygen uptake by Streptococcus cremoris was observed when H2O2 and SCN- were present in equimolar amounts and the pH was below 6.0 (Modi et al., 1991). Fluoride (F-) ions at concentrations present in vivo at the plaque/enamel interface (0.05-10 mM) inhibit the activities of LP, myeloperoxidase and total salivary peroxidase in a pH- and dose-dependent manner (Hannuksela et al., 1994). Furthermore, the generation of antimicrobial products in vivo, hypothiocyanite (HOSCN/OSCN-), of the oral peroxidase systems was inhibited by F-, again at low pH (5.0-5.5) both in buffer (by 45%) and in saliva (by 15%). Small molecular weight media components in brain-heart infusion broth could also interfere with the antimicrobial activity of LP (Hoogendorn & Moorer, 1973). D. Resistance Several strains of Streptococcu cremoris demonstrate a low degree of susceptibility to the antimicrobial effects of LP system. Extracts from a resistant strain were able to reverse the inhibition of a susceptible strain. It was suggested that the resistant strains utilize an NADH2-oxidizing enzyme to catalyze the oxidation of NADH2 by OSCN-, and thereby lower the inhibitory levels (Oram & Reiter, 1966a). Under aerobic conditions, certain strains of S. agalactiae develop a cyanide-sensitive respiratory system resistant to LP/SCN- (Mickelson, 1979). Carlsson and co-workers (1983) reported that Streptococcus mitis and Streptococcus sanguis, but not Streptococcus salivarius or S. mutans, had a high capacity for recovering from inhibition by OSCN-. This resistance is due to the presence of a streptococcal oxidoreductase that catalyzes the reduction of OSCN- to SCN-. The activity of this enzyme was much higher in S. mitis and S. sanguis than in S. salivarius and S. mutans. The relative resistance of these organisms to OSCN- was suggested due to relative difference in activity of this oxidoreductase enzyme. Hoogendoorn (1976) suggested the potential role of NADPH in S. mutans resistance to the LP/SCN-. The inhibited streptococcal cells possibly recover by utilizing NADPH to reduce the compounds oxidized by OSCN-. When NADPH levels are exceeded by H2O2 (from which OSCN- is generated), streptococci fail to reverse the antimicrobial effects of LP/SCN-. Resistance of oral bacteria to OSCN- inhibition seems to correlate with their peroxidogenicity (Mansson-Rahemtulla et al., 1982). Thomas and co-workers (1983) identified three major types of peroxide-generating S. mutans, Class-I strains produced large amounts of H2O2; Class-II produced moderate amounts of H2O2; and Class-III produced little H2O2 or none. Class I and class II strains were auto-inhibited due to the utilization of streptococcal H2O2 by LP/SCN- to generate antimicrobial OSCN-. Among Class-I and -II strains the H2O2 and OSCN- accumulation increased with culture age. Detectable H2O2 was excreted by class III cells but did not accumulate due to the high levels of peroxide-reducing enzymes present in these strains. However, cells of all classes were inhibited by the LP/SCN- when H2O2 was added exogenously. Preincubation of cells with glucose and with certain sulfhydryl compounds could lead to elevated cell sulfhydryl content and to increased resistance (Thomas et al., 1983). A two-step mechanism to elucidate LP/SCN- resistance was suggested. The first step pos© 2000 by CRC Press LLC
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tulates a reductase-dependent NADPH generation of sulfhydryl compounds from intracellular disulfides. In the second step, these sulfhydryl compounds rapidly reduce OSCNto SCN- in an enzyme-independent reaction. The net result is an NADPH-dependent reduction of OSCN- to SCN- with conservation of intracellular sulfhydryl concentration.
VI. ANTIMICROBIAL SPECTRUM The LP system could elicit stasis and/or cidal activity on a variety of susceptible microorganisms including bacteria, fungi, viruses and parasites (TABLE 2). The molecular mechanism(s) of such inhibitory effects depend on the type of electron donor, test media, temperature, pH, etc. and could range from oxidative killing to blockade of glycolytic pathways or interference in cytopathic effects (FIGURE 2). A. Antibacterial effects In 1894, Hesse found that gram-negative, catalase-positive species of Vibrio and Salmonella were killed in raw milk. Gram-negative bacteria seem to be more easily killed than are gram-positive cells by extended incubation with OSCN-, especially at low temperatures. The pH-dependence of killing also seems to be greater for gram-negative species. E. coli and S. typhimurium are difficult to kill above pH 7.0 and at temperatures over 20ºC, when SCN- is the electron donor. However, under similar conditions, a cidal activity could be achieved with I- as electron donor. Both SCN- and I- promote killing by the LP system when incubated with bacteria at pH 5.5 or less and at 0-5ºC (Pruitt & Reiter, 1985). The inner membrane of gram-negative bacteria appears to be more extensively damaged by LP treatment than is that of gram-positive species (Marshall & Reiter, 1980). LP present in various secretions oxidizes SCN- in the presence of H2O2 to an unstable oxidation product (OSCN-), which is bactericidal for enteric pathogens including multiple antibiotic resistant strains of E. coli. The system damages the inner membrane causing leakage and cessation of uptake of nutrient, leading eventually to death of the organisms and lysis. The antimicrobial activity of LP/H2O2/SCN- system against E. coli seems related to the oxidation of bacterial sulfhydryls (Thomas & Aune, 1978). LP catalyzed oxidation of SCN- results in accumulation of OSCN-. A portion of the bacterial sulfhydryls was oxidized by OSCN- to yield sulfenic acid and sulfenyl thiocyanate derivatives. The remaining sulfhydryls were not oxidized, although OSCN- was present in large excess. The oxidation of sulfhydryls to sulfenyl derivatives inhibits bacterial respiration. Adding sulfhydryl compounds to reduce the sulfenyl derivatives and the excess OSCN- could reverse this inhibition. Also, the removal of excess unreacted OSCN- by washing cells could reverse this inhibition. After washing, the bacteria demonstrated a time-dependent recovery of their sulfhydryl content and resulted in cellular restoration of the ability to respire. The inhibited cells were viable if diluted and plated shortly after the incubation with the LP/H2O2/SCN- system. On the other hand, long-term incubation in the presence of the excess OSCN- results in loss of viability. Also, the inhibition of respiration is irreversible. During this long-term incubation, the excess OSCN- was consumed and the sulfenyl derivatives disappear. The LP/SCN-/H2O2 system could inhibit the growth of enterotoxigenic E. coli strains that cause scouring in neonatal and post-weaning piglets (Grieve et al., 1992). An enzymatic system for H2O2 generation (glucose oxidase; 0.1 U/ml) and a chemical source © 2000 by CRC Press LLC
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TABLE 2: Antimicrobial activity of lactoperoxidase system Microorganism
Donor
H2O2 source
Inhibitory effect
Reference
Gram +ve bacteria Bacillus cereus B. megatherium Lactobacillus casei L. acidophilus L. plantarum L. bulgaricus L. helvaticus L. jugurti Sarcina lutea Staph. albus Staph. aureus Strep. cremoris S. lactis S. pyogenes S. agalactiae
SCNSCNSCNISCNSCN-
Reagent Reagent Bacteria Bacteria Bacteria Bacteria
Collagenase production Stasis Stasis Lysine accumulation Stasis Acid production
Tenovuo et al., 1983 Klebanoff et al., 1966 Iwamoto et al., 1972 Zeldow, 1963 Hogendron & Moorer, 1973 Portman et al., 1962
SCNSCNI- or SCNMilk/ SCNSCNMilk Milk/ SCN-
Reagent Reagent S. mitis Bacteria Reagent Bacteria
S. fecalis S. mitis S. mutans S. salivarius S. sanguis
SCNSCNSCNSCNSCN-
Bacteria Reagent Bacteria Reagent Bacteria
Stasis Stasis Amino acid uptake Glycolysis Stasis Cidal / production Lactic acid production Sugar transport Stasis Peroxide excretion Sugar uptake Acid production Stasis / acid production
Reiter, 1978 Klebanoff et al., 1966 Harmon & Klebanoff, 1973 Reiter et al., 1963 Marshall & Reiter, 1980 Mickelson, 1979 Brown & Mickelson, 1979 Mickelson, 1977 Klebanoff et al., 1966 Carlsson et al., 1983 Thomas et al., 1983 Carlsson et al., 1983 Carlsson et al., 1983
L. pneumophila S. typhimurium
SCNIWhey Milk ClSCN-
P. aeruginosa
SCN-
P. fluorescens
Milk/ SCN-
Reagent Reagent Oxidase Reagent Reagent Oxidase Reagent Oxidase Reagent Oxidase Reagent
Stasis Stasis Amino acid uptake Stasis Cidal Cidal Cidal / stasis Cidal Cidal Cidal Cidal
Klebanoff et al., 1966 Klebanoff, 1967 Harmon & Klebanoff, 1973 Stephens et al., 1979 Lochner et al., 1983 Reiter et al., 1976 Purdy et al., 1983 Reiter et al., 1976 Pruitt & Reiter, 1985 Björck et al., 1975 Björck, 1978
IISCN-
S.mitis Reagent Oxidase
Cidal Cidal Stasis
Harmon & Klebanoff, 1973 Lehrer, 1969 Popper & Knorr, 1997
I- / Br-
Reagent
Cidal
Belding & Klebanoff, 1970
SCNSCN-/I-
Reagent Oxidase
Delay/loss of cytopathy Cell infectivity
Courtois et al., 1990 Yamaguchi et al., 1993
Gram -ve bacteria Escherichia coli
Fungi Candida tropicalis Candida albicans Rhodotorula rubra Sacch. cerevisiae Aspergillus niger Byssochlamys fulva Viruses Polio virus Vaccinia virus HSV-1 HIV-1
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FIGURE 2: Antimicrobial spectrum of lactoperoxidase system. (i) Bacillus cereus growth was inhibited by 250 mU/ml LP and 1 mM I- in the presence of H2O2 either at 0.1 mM (!) or 0.2 mM (O) concentration compared to the control ( ) (adapted from Tenovuo et al., 1985). (ii) Salmonella typhimurium rough mutant TA1535 growth in LP system containing 300 µM OSCN- either with 50 µg/ml of catalase (") or without catalase (O) and compared to control (!) (adapted from Purdy et al., 1983). (iii) Cidal effects of LP system against Escherichia coli in the presence of SCN- at concentrations of 0.15 mM (#) or 0.30 mM ( ); also against Pseudomonas aeruginosa with SCN- at concentrations of 0.15 mM (!) or 0.30 mM (O) (adapted from Reiter et al., 1976). (iv) Listeria monocytogenes survival curves at 57.8 °C in milk (O), in milk containing 0.6 mM H2O2 (!) and milk containing lactoperoxidase system, 2.4 mM SCN- / 0.6 mM H2O2 / 9.2 µg of inherent LP/ml ($) (adapted from Kamau et al., 1990).
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(sodium carbonate peroxyhydrate; 90 mg/L) were used in the LP system to test 19 strains in a 6-h growth assay at 37ºC. Only three strains were highly sensitive to the LP/glucose oxidase system, while all showed marked growth inhibition with the LP/peroxyhydrate system. H2O2 alone had less effect than the complete system. The interaction between milk xanthine oxidase and LP in a model system and antimicrobial action of these enzymes on E. coli O111 was reported (Al’perovich et al., 1992). Bacterial superoxide dismutase (SOD), which transforms O2-. (reaction product of xanthine oxidase) into H2O2 was necessary for the reaction. It was suggested that the combination of these enzymes possibly protect neonates against intestinal infections. Bacterial SOD could act as the key factor, creating the antimicrobial LP system. Antimicrobial activity of LP system against verotoxigenic E.coli O157:H7 has also been reported (Heuvelink et al., 1998). The LP/SCN-/H2O2 system exerts both bacteriostatic and bactericidal activities against strains of S. typhimurium (Purdy et al., 1983). The bactericidal activity is dependent on the permeability of the bacterial cell envelope. The deep rough mutant TA1535, with the most permeable cell envelope, is killed both at neutral and acid pH, whereas very little or no killing is observed with the intact cells of the wilds-type parent strain. The delta gal mutant, TA1530, representing an intermediate in cell envelope permeability, is inhibited to a much lesser extent than TA1535. Bacteria in log phase of growth are more sensitive to the bactericidal effects than are those in stationary phase. Growth phase has little influence on the bacteriostatic effects. The wild-type strain produced significant quantities of acid in the presence of glucose. This acid production is inhibited by the LP/SCN/H2O2 system. In contrast, this inhibition is not reversed by addition of a reducing agent (2-mercaptoethanol) in several strains of streptococci. The inhibition of Bacillus cereus by LP and myeloperoxidase antimicrobial systems was reported (Tenovuo et al., 1985). With the LP/SCN-/H2O2 system, the growth inhibition is directly proportional to the amount of OSCN- ions present. This inhibition is associated with reduced extracellular release of collagenase activity from the cells. With LP, the antimicrobial efficiency of the oxidizable substrates SCN- is greater than I-, and with myeloperoxidase, the efficiency was I- greater than Cl- greater than SCN-, respectively. LP failed to oxidize Cl-. The LP/SCN-/ H2O2 system consisting of LP (0.37 U/ml), KSCN (0.3 mM), and H2O2 (0.3 mM), delayed but did not prevent growth of Listeria monocytogenes at 30ºC in broth and at 20ºC in milk (Siragusa & Johnson, 1989). LP (10-200 µg/ml) could elicit significant reduction of S. mutans adherence to hydroxyapatite in a dose-dependent manner (Roger et al., 1994). The strongest inhibition of adhesion was found when both saliva-coated apatite and bacteria were pretreated with LP. The inhibition of adherence of a serotype c strain of S. mutans to saliva-coated hydroxyapatite is a novel antibacterial mechanism for LP. Stephens and co-workers (1979) examined the LP activity in milk of sows suckling piglets infected with E. coli. A 5-fold increase of LP activity in milk was observed during the 3-4 weeks of lactation. The antibacterial activity of milk from sows suckling normal young increased with the LP, and this bactericidal activity could be reversed by LP inhibitors such as penicillamine and cysteine but not by iron supplementation to saturate the lactoferrin. In milk from sows suckling infected young, bacteriostatic activity was observed in 14 days after infection and needed iron or both iron and penicillamine (or cysteine) for reversal, indicating the role of both the antibody-lactoferrin and the LP systems. © 2000 by CRC Press LLC
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In vivo antimicrobial activation of the LP system (LP/SCN-/ H2O2) in the calf abomasum was reported (Reiter et al., 1980). Milk provided the two essential factors, namely the LP and the SCN-, while the third factor was rendered either by an H2O2 generating system (glucose oxidase and glucose) or by H2O2-producing lactobacilli (natural gut flora in the abomasum of the calf). Marshall and co-workers (1986) suggested an important role for the LP/SCN/H2O2 system in protecting lactating mammary glands from Streptococcus uberis infections. However, this protective barrier seemed to be ineffective as the involution progressed. Products of SCN- oxidation by LP could inhibit peroxide producing gram-positive bacteria. Such products demonstrate cidal activity against gram-negative bacteria including Pseudomonas spp. and E. coli (Bjorck et al., 1975). The LP system could inhibit most strains of lactobacilli and streptococci; however, the sensitivity varies from strain to strain. Exposure of susceptible cells to the LP system could cause a rapid (200 calves). Calves are susceptible to scour (diarrhea) early in life, particularly during transfers to large calf units. Scouring is either dietary when milk replacers are used or caused by infection with E. coli or viruses. Depending on the severity and period of infection, afflicted animals lose weight, are retarded in growth development and may die. Reiter and co-workers (1981) demonstrated that feeding of LP supplemented milk could prevent incidence of scouring in calves and also improve weight-gain in LP-treated animals. The clinical efficacy of a preparation based on the LP system and lactoferrin was tested in calves experimentally infected with enterotoxigenic E. coli (Still et al., 1990). Mortality, occurrence and duration of diarrhea were significantly lower (P caffeic acid > tyrosol (approximate EC50 values: 15, 80, 200, and 500 µM, respectively). In contrast, none of these compounds caused substantial inhibition of thromboxane generation via the cyclo-oxygenase pathway. Hydroxytyrosol, caffeic acid, oleuropein, and tyrosol (decreasing order of effectiveness) also quenched the chemiluminescence signal due to reactive oxygen species generated by phorbol myristate acetate-stimulated rat leukocytes. None of these compounds were toxic to leukocytes at the concentrations tested. The authors have concluded that the phenolics found in virgin olive oil possess an array of potentially beneficial lipoxygenase-inhibitory, prostaglandin-sparing, and antioxidant properties. Saenz et al. (1998) have tested oleuropein, tyrosol, squalene and the fraction of sterols and triterpenoid dialcohols from the unsaponifiable fraction obtained from virgin olive oil for possible cytostatic activity against McCoy cells, using 6-mercaptopurine as a positive control. Samples of sterols and triterpenic dialcohols showed a strong activity. B. Oleoresins 1. Antimicrobial activity. Conner and Beuchat (1984) reported that an oleoresin of cinnamon was extremely inhibitory against eight yeasts, i.e. Candida lipolytica, Debaryomyces hansenii, Hansenula anomala, Kloeckera apiculata, Lodderomyces elongisporus, Rhodotorula rubra, S. cerevisiae, and Torulopsis glabrata. Essential oil of clove dispersed (0.4% v/v) in a concentrated sugar solution, had a marked germicidal effect against various bacteria and C. albicans (Briozzo, et al., 1989). S. aureus (five strains), Klebsiella pneumoniae, P. aeruginosa, Clostridium perfringens, and E. coli inoculated at a level of 107 cfu/ml, and C. albicans (inoculum 4.0 x 105 cfu/ml) were killed (>99.9%) after 2-7 min in broth supplemented with 63% (v/w) of sugar, and containing 0.4% (v/w) of essential oil of clove. Presence of organic matter (i.e. human or bovine serum) did not impair its antimicrobial activity. Sugar was not necessary for the antimicrobial activity of clove oil, but the concentrated sugar solution provided a good vehicle for obtaining uniform oil dispersion that is relatively stable for certain practical applications. 2. Multifunctionality. The oleoresin from Brazilian Copaifera species yielded copalic acid and sesquiterpenes and showed marked anti-inflammatory activity (Basile et al., 1988). The oleoresin significantly inhibited carageenan-induced pedal edema following oral doses from 0.70 to 2.69 ml/kg, but was somewhat less effective than 50 mg/kg calcium phenylbutazone. Repeated administration of the oleoresin at a dose of 1.26 ml/kg for a 6-day period reduced granuloma formation with a response comparable to that of 20 mg/kg of calcium phenylbutazone. This same dose of oleoresin also reduced the vascular permeability to intra-cutaneous histamine. The LD50 value of the oleoresin in rats was estimated to be 3.79 (3.21-4.47) ml/kg. Consumption of carotenoids has frequently been inversely correlated with cancer incidence. Sharoni and co-workers (1997) have used the 7,12-dimethylbenz[a]anthracene (DMBA)-induced rat mammary tumor model to compare the effect of
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lycopene-enriched tomato oleoresin on the initiation and progression of these tumors with that of β-carotene. Rats were injected i.p. with lycopene-enriched tomato oleoresin or βcarotene (10 mg/kg, twice per week) for 2 weeks prior to tumor induction by DMBA and for an additional 16 weeks after carcinogen administration. HPLC analysis of carotenoids extracted from several tissues showed that both carotenoids were absorbed into blood, liver, mammary gland, and mammary tumors. The tomato oleoresin-treated rats developed significantly fewer tumors, and the tumor area was smaller than that of the unsupplemented rats. Rats receiving β-carotene showed no protection against the development of mammary cancer. In vitro studies on the effect of alcoholic extracts of turmeric, turmeric oil and turmeric oleoresin (TOR), on the incidence of micronuclei (MN) in lymphocytes from normal healthy subjects showed that the test compounds did not cause any increase in the number of MN as compared with those found in untreated controls (Hastak et al., 1997). Further it was observed that all three compounds offered protection against benzo[a]pyrene induced increase in MN in circulating lymphocytes. In subsequent studies, patients suffering from submucus fibrosis were given a total oral dose of TO (600 mg turmeric oil mixed with 3 g turmeric/day). TOR (600 mg + 3 g turmeric/day) and 3 g turmeric/day as a control for 3 months. It was observed that all three treatment modalities decreased the number of micronucleated cells both in exfoliated oral mucosal cells and in circulating lymphocytes. TOR was found to be more effective in reducing the number of MN in oral mucosal cells, but in circulating lymphocytes the decrease in MN was comparable in all three groups. C. Thymol and carvacrol The antimicrobial activity of oregano and thyme has been attributed to their essential oils which contain the terpenes: carvacrol [2-methyl-5-(1-methylethyl)phenol] and thymol [5-methyl-2-(1-methylethyl)phenol], respectively. 1. Antimicrobial effects. Katayama and Nagai (1960) tested thymol and carvacrol against Bacillus subtilis, Salmonella Enteritidis, S. aureus, Pseudomonas aeruginosa, Proteus and E. coli and found inhibition of all microorganisms at dilutions as low as 1:2000. Essential oil from oregano had the highest activity of a number of essential oils tested against both fungi and bacteria (Maruzella & Henry, 1958; Maruzella & Liguori, 1958). Ting and Deibel (1992) determined the MIC of oregano against Listeria monocytogenes at 24˚C in a microbiological medium to be 0.5-0.7% w/v. Oregano at 0.5% or 1.0% was bacteriostatic to L. monocytogenes in trypticase soy agar at 4 or 24˚C but had little effect growth of the microorganism in beef at 1.0% (Ting & Deibel, 1992). Growth and lactic acid production of Lactobacillus plantarum and Pediococcus cerevisiae were inhibited by 4 mg/ml oregano for 7 days (Zaika & Kissinger, 1981). Lower concentrations of the spice stimulated acid production. Rosemary, sage and thyme inhibited the microorganisms to a lesser extent than oregano but also caused stimulation of acid production (Zaika et al., 1983). Kim et al. (1995) evaluated the antibacterial activity of essential oil constituents against E. coli, E. coli O157:H7, Salmonella Typhimurium, L. monocytogenes, and Vibrio vulnificus at 5, 10, 15, and 20% using disk and dilution assays. Carvacrol showed strong bactericidal activity against all strains, while limonene, nerolidol, and β-ionone were mostly inactive. Carvacrol was highly bactericidal at 250 µg/ml
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TABLE 4. Minimum lethal concentrations (µg/ml; ≥ 99.9% decrease in viability) of thymus essential oil and its components against various bacteria and yeasts. Microorganism
Thyme oil M.L.C. Range
Active Component
Component M.L.C (µg/ml)
Gram-negative bacteria Escherichia coli Escherichia coli O157:H7 Pseudomonas aeruginosa Salmonella Typhimurium Yersinia enterocolitica
450-900 450-900 >900 450-900 450-900
Thymol / Carvacrol Carvacrol Thymol Thymol / Carvacrol
225 225 56.25 225
Gram-positive bacteria Bacillus cereus Listeria monocytogenes Staphylococcus aureus
225-900 225-900 225-900
Thymol Thymol / Carvacrol Thymol
450 450 225
Yeasts Candida albicans Saccharomyces cerevisiae
225-400 225-400
Thymol / Carvacrol Thymol / Carvacrol
112.5 112.5
Adapted from Cosentino et al. (1999)
against Salmonella Typhimurium and Vibrio vulnificus. Pol and Smid (1999) reported that carvacrol enhanced the antimicrobial activity of nisin against growth of both Bacillus cereus and L. monocytogenes. Karapinar and Aktug (1986) determined the inhibitory activity of thyme, mint, and bay leaves on growth of Salmonella Typhimurium, S. aureus and Vibrio parahaemolyticus. Thyme was the most effective antimicrobial of the spices and bay leaves the least active. Vibrio parahaemolyticus was the most sensitive bacteria and Salmonella Typhimurium the most resistant. Beuchat (1976) also showed that oregano and thyme were bactericidal to Vibrio parahaemolyticus at 0.5% as whole spices and bacteriostatic at 100 µg/ml as essential oils. Firouzi et al. (1998) found that thyme essential oil was the most effective antimicrobial against L. monocytogenes 4b growth compared to a number of other spice and herb extracts. Cosentino et al. (1999) reported on the composition and antimicrobial activity of thyme from different sources. They found that the composition of the essential oil of thymus varied greatly. Among the four samples analyzed, all of which were from Sardinia, the major component in all was thymol (29-50%) followed by variable amounts of carvacrol, p-cymene and α-pinene. The researchers then determined the minimum lethal concentration of the essential oil and components of the essential oil against various bacteria and yeasts (TABLE 4). While thymol and carvacrol were the most active components of the essential oils, the activity varied depending upon the source and the type of microorganism. Cosentino et al. (1999) suggested that components of the essential oil may have acted synergistically (e.g., thymol and carvacrol) or antagonistically (e.g., p-cymene) with other components to alter overall antimicrobial effectiveness. Juven et al. (1994) evaluated thyme essential oil and its components against Salmonella Typhimurium to determine their activity and assess the interactions of environmental factors on antimicrobials activity. They first determined that 175 µg/ml or 225 µg/ml thymol or carvacrol, respectively, completely inhibited Salmonella Typhimurium recovery under aerobic or anaerobic conditions. p-Cymene up to 500 µg/ml had no effect on the microorganism. Factors reducing the activity of thymol included presence of Tween 80, aerobic incubation, reduced pH and presence of bovine serum albumin.
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TABLE 5. Minimum inhibitory concentrations (% v/v) of selected essential oils of herbs and spices against various bacteria and yeasts as determined by agar dilution. Spice Basil Bay Black pepper Clove Coriander Fennel Ginger Lemongrass Marjoram Oregano Peppermint Rosemary Sage Spearmint Tea tree Thyme Wintergreen
Enterococcus faecalis
E. coli
Pseudomonas aeruginosa
Salmonella Typhimurium
S. aureus
Candida albicans
>2.0 0.5 1.0 0.5 0.25 >2.0 >2.0 0.12 2.0 0.25 2.0 >2.0 2.0 2.0 2.0 0.5 >2.0
0.5 0.12 >2.0 0.25 0.25 0.5 >2.0 0.06 0.25 0.12 0.5 1.0 0.5 0.25 0.25 0.12 0.5
>2.0 1.0 >2.0 >2.0 >2.0 >2.0 >2.0 1.0 >2.0 2.0 >2.0 >2.0 >2.0 >2.0 >2.0 >2.0 >2.0
2.0 0.25 >2.0 >2.0 1.0 1.0 >2.0 0.25 0.5 0.12 1.0 >2.0 2.0 0.5 0.5 >2.0 0.5
2.0 0.25 >2.0 0.25 0.25 0.25 >2.0 0.06 0.5 0.12 1.0 1.0 1.0 0.25 0.5 0.25 2.0
0.5 0.12 >2.0 0.12 0.25 0.5 >2.0 0.06 0.25 0.12 0.5 1.0 0.5 0.12 0.5 0.12 0.25
Adapted from Hammer et al. (1999a)
Hammer et al. (1999a) found that the method for determining antimicrobial effectiveness of essential oils may have a significant effect on identifying active components. For example, they showed that, using an agar dilution assay, the most effective of 52 spice and herb essential oils and plant extracts against a variety of bacteria and a yeast were lemongrass, oregano and bay (TABLE 5). Little activity was demonstrated for thyme. However, when a different assay was used, such as the broth micro-dilution assay, thyme was the most effective essential oil among 20 herbs, spices and plant extracts tested against E. coli, S. aureus and Candida albicans (TABLE 6). This shows that the type of assay may influence the results of antimicrobial activity analyses. Similar results were demonstrated by Kubo et al. (1991), who found no inhibition of selected microorganisms with a series of volatile components from cardamom using a disk diffusion assay but significant inhibition using a broth dilution assay. In contrast, Hao et al. (1998) found no antimicrobial activity by thyme against Aeromonas hydrophila or L. monocytogenes in cooked beef. This could have been due to interference from food components, especially lipids. Both growth and aflatoxin production of A. parasiticus were inhibited by 500 µg/ml thymol for 10 days at 28°C (Buchanan & Sheperd, 1981). At 100 µg/ml, thymol nearly eliminated aflatoxin production by the mold. Conner and Beuchat (1984) tested 32 essential oils from spices and plant extracts at 1 and 10% for growth inhibition activity against 13 different yeast species. The most active growth inhibitors were oregano and thyme followed by clove and cinnamon. Karapinar (1985) confirmed that thyme was an effective inhibitor of Aspergillus parasiticus growth. Aqueous and ethanolic extracts of Thymus capitatus (10-200 mg/ml), saponin, resin and essential oil of the plant (10-5000 µg/ml) inhibit the growth of several bacteria and fungi (Kandil et al., 1994). The essential oil of thyme or its constituent thymol, especially under anaerobic conditions reduce the viable counts of Salmonella Typhimurium (Juven et al., 1994). Antagonistic effects of thymol against S. aureus were also greater
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TABLE 6. Comparison of minimum inhibitory concentrations (% v/v) of essential oils of herbs and spices against Escherichia coli, Staphylococcus aureus and Candida albicans in agar dilution (AD) and broth micro-dilution (BD) assays. Spice
Escherichia coli
Bay Clove Ginger Lemongrass Peppermint Thyme
AD 0.12 0.25 >2.0 0.06 0.5 0.12
BD 0.12 0.12 >4.0 0.12 0.12 0.03
Staphylococcus aureus AD 0.25 0.25 2.0 0.06 1.0 0.25
BD 0.12 0.12 >4.0 0.06 .012 0.03
Candida albicans AD 0.12 0.12 >2.0 0.06 0.5 0.12
BD 0.06 0.12 >4.0 0.06 0.12 0.03
Adapted from Hammer et al. (1999a)
under anaerobic conditions. In contrast to the phenolic constituents, the chemically related terpenes p-cymene and γ-terpinene had no antagonistic effects against Salmonella Typhimurium. The addition of Desferal counteracted the antibacterial effects of both thyme oil and thymol, however, any possible role of iron in the oxygen-related antibacterial action was not established. In the presence of thymol, the viable counts of Salmonella Typhimurium obtained on a minimal medium were lower than those obtained on nutrient agar. Addition of bovine serum albumin (BSA) neutralized the antibacterial action of thymol, suggesting that the effects of BSA or Desferal are due to their ability to bind phenolic compounds through their amino and hydroxylamine groups, respectively, thus preventing complexation reactions between the oil phenolic constituents and bacterial membrane proteins. This hypothesis was supported by the marked decrease in the viable counts of Salmonella Typhimurium caused by either thyme oil or thymol when the pH of the medium was changed from 6.5 to 5.5 or the concentration of Tween 80 in the medium was reduced. The antifungal activity of several components of essential oils structurally related to eugenol were evaluated using a paper-disk method (Pauli & Knobloch, 1987). Equimolar amounts were tested on more than ten fungal strains known to contaminate food. Iso-eugenol, cinnamaldehyde, carvacrol, eugenol and thymol revealed the strongest antifungal activity. The most resistant strain appeared to be Penicillium verrucosum var. cyclopium, and the most sensitive was P. viridicatum. Some of the structural effects were considered, including a free hydroxyl group in connection with an alkyl substituent which seemed to represent an especially active configuration of phenolic compounds and which rendered antimicrobial activity. The inhibitory effects of 10 selected Turkish spices, oregano essential oil, thymol and carvacrol towards growth of 9 foodborne fungi were investigated in culture media at pH 3.5 and 5.5 (Akgul & Kivanc, 1988). The antifungal effects of sodium chloride, sorbic acid and sodium benzoate and the combined use of oregano with sodium chloride were also tested under the same conditions for comparison. Of the spices tested, only oregano at 1.0, 1.5, 2.0% (w/v) levels showed effect on all fungi. 8% (w/v) sodium chloride was less effective than oregano. Oregano essential oil, thymol or carvacrol at concentrations of 0.025% and 0.05% completely inhibited the growth of all fungi, showing greater inhibition than sorbic acid at the same concentrations. The combined use of oregano and sodium chloride exhibited a synergistic antifungal effect. Organic and aqueous solvent extracts and fractions of the plant Micromeria nervosa (Labiatae) consists of carvacrol and thymol as main ingredients. These extracts strongly inhibit Candida albicans and various bacteria including Proteus vulgaris, Pseudomonas aeruginosa (Ali-Shtayeh et al., 1997). © 2000 by CRC Press LLC
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2. Antioxidant effects. Antioxidants minimize oxidation of the lipid components in foods. There is an increasing interest in the use of natural and/or synthetic antioxidants in food preservation, but it is important to evaluate such compounds fully for both antioxidant and pro-oxidant properties. The antioxidant properties of thymol, carvacrol, 6ginerol, hydroxytyrosol and zingerone are well characterized (Aeschbach et al., 1994). These monoterpenoids decrease peroxidation of phospholipid liposomes in the presence of iron(III) and ascorbate, however, zingerone has only a weak inhibitory effect on the system. The compounds were good scavengers of peroxyl radicals (CCl3O2; calculated rate constants > 106 M/sec) generated by pulse radiolysis. Thymol, carvacrol, 6-gingerol and zingerone were not able to accelerate DNA damage in the bleomycin-Fe(III) system. Hydroxytyrosol promoted deoxyribose damage in the deoxyribose assay and also promoted DNA damage in the bleomycin-Fe(III) system. This promotion was inhibited strongly in the deoxyribose assay by the addition of BSA to the reaction mixtures. These data suggest that thymol, carvacrol and 6-gingerol possess useful antioxidant properties and may become important in the search for ‘natural’ replacements for ‘synthetic’ antioxidant food additives. 3. Therapeutic effects. The antimicrobial action of thymol-camphor against S. aureus was compared with 21 pharmaceutical preparations in vitro and was found superior (Trebitsch, 1978). The essential oil of Bupleurum fruticosum was investigated qualitatively and quantitatively together with the anti-inflammatory activity of the whole essential oil and its major components (Lorente et al., 1989). In addition, antispasmodic activity was determined in rat uterus preparations using acetylcholine and oxytocin as agonists. The anti-inflammatory activity shown by the essential oil was attributed to α-pinene and β-pinene, and the presence of thymol and carvacrol as minor components, have potentiated the action of these hydrocarbons. Didry et al. (1993) have tested the antimicrobial activity of thymol, carvacrol and cinnamaldehyde against bacteria involved in upper respiratory tract infections. The broad spectrum of activity and the synergistic effect observed with some combinations (specially thymol and carvacrol) could allow the use of the three compounds alone or, like thymol an carvacrol, combined during the treatment of respiratory infections. Thymol and carvacrol, as the essential oils of two labiatae plants, Mosla chinensis Maxim. and Pogostemon cablin Benth were shown to elicit antibacterial activity against periodontopathic bacteria, including Actinobacillus, Capnocytophaga, Fusobacterium, Eikenella and Bacteroides species. (Osawa et al., 1990). Didry et al. (1994) have also tested the antimicrobial activity of thymol, carvacrol, cinnamaldehyde and eugenol alone or combined on eight oral bacteria. The compounds inhibited seven microorganisms and a synergistic effect was observed with certain combinations. The four compounds were suggested for therapeutic applications alone or in combination, as eugenol and thymol, eugenol and carvacrol, thymol and carvacrol, during the treatment of oral infectious diseases. Antimicrobial effects of thymol on oral pathogens Porphyromonas gingivalis, Selenomonas artemidis and Streptococcus sobrinus were reported (Shapiro & Guggenheim, 1995). The extremely rapid efflux of intracellular constituents evoked by thymol is consistent with its postulated membrane-tropic effects. Correlations between leakage-inducing concentrations of thymol and MIC and minimal bactericidal concentrations suggest that membrane perforation is a principal mode of
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action of this substance. The thymol-induced decline in intracellular ATP in S. sobrinus appears to be entirely attributable to leakage, whereas in P. gingivalis thymol may also inhibit ATP-generating pathways. Relative changes in the transmembrane potential of resting cells of S. sobrinus pulsed with glucose are as sensitive to thymol as is leakage from this organism. The effects of thymol on transmembrane potential are probably secondary to those arising from leakage of intracellular substances. In vitro leishmanicidal and trypanocidal activities of a petroleum ether extract of Oxandra espintana have been investigated (Hocquemiller et al., 1991). Four aromatic monoterpenes were isolated, of which two are novel: espintanol, responsible for the antiparasite activity, and O-methylespintanol. Espintanol was tested in vitro on 20 strains of Trypanosoma cruzi and 12 strains of Leishmania spp. Its structure was determined by spectroscopic methods and confirmed by its preparation starting from carvacrol. Thymol and carvacrol are also shown to inhibit Cryptococcus neoformans, an opportunistic fungal pathogen in AIDS patients. The MIC was 100-200 µl/L in vitro (Viollon & Chaumont, 1994). Thymol and carvacrol are also the main essential oil components of Lippia sidoides Cham. These essential oils show antibacterial and antifungal properties against microorganisms on the skin of feet and armpits (Lacoste et al., 1996). These essential oils elicit strong antagonistic activities against Corynebacterium xerosis that contributes to axillary odor. D. Borneol The active antimicrobial fraction of sage and rosemary has been suggested to be borneol and other phyto-phenols of the terpene fraction. At 2% in bacterial growth medium sage and rosemary were more active against Gram-positive than Gram-negative strains (Shelef et al., 1980). The inhibitory effect of these two spices at 0.3% was bacteriostatic while at 0.5% they were bactericidal to the Gram-positive strains. Pandit and Shelef (1994) studied the antimicrobial effectiveness of 18 spices against the growth of L. monocytogenes in culture medium. The most effective compound was 0.5% rosemary which was bactericidal. The fraction of rosemary essential oil that was most inhibitory to L. monocytogenes was α-pinene. Smith-Palmer et al. (1998) demonstrated that rosemary (0.02-0.05%) and sage (0.02-0.075%) were inhibitory to Gram-positive L. monocytogenes and S. aureus but not to Gram-negative bacteria. Further, Pandit and Shelef (1994) showed that L. monocytogenes Scott A growth in refrigerated fresh pork sausage was delayed by 0.5% ground rosemary or 1% rosemary essential oil. In contrast, Mangina and Muyima (1999) indicated little antimicrobial activity with essential oil of rosemary against bacteria and yeast in an agar diffusion assay. They found that, with a 1:2 dilution of the oil, 25 of 29 bacterial strains and 10 of 12 yeast strains tested showed zones of inhibition about 3.5 mm. The lack of activity could be due to the assay utilized. Shelef et al. (1984) found that sensitivity of Bacillus cereus, S. aureus and Pseudomonas to sage was greatest in microbiological medium and significantly reduced in rice and chicken and noodles. It was theorized that loss of activity was due to solubilization of the antimicrobial fraction in the lipid of the foods. Hefnawy et al. (1993) evaluated 10 herbs and spices against two strains of L. monocytogenes in tryptose broth. The most effective spice was sage which at 1% decreased viable L. monocytogenes by 5-7 logs after 1 day at 4°C. Allspice was next most effective inactivating the microorganism in 4 days.
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Hammerschmidt et al. (1993) analyzed the essential oils of the aerial parts of Jasonia candicans and J. montana by gas chromatography-mass spectrometry (GC/MS). Of twenty-one components identified in the volatile oil of J. candicans, intermediol was the main constituent. Fifty-eight components were characterized in the essential oil of J. montana. Borneol, bornyl acetate, camphor, chrysanthemol, intermediol, and 1,8-cineole were the major constituents in this oil. The two oils showed antibacterial activity against Bacillus subtilis. They also showed a marked antifungal activity against Trichophyton mentagrophytes, Cryptococcus neoformans, and Candida albicans. Liu (1990) reported the therapeutic effects of borneol. In a clinical trial, 170 patients with purulent otitis media were treated with borneol-walnut oil of various concentrations, and the controls (108 patients) were treated with neomycin. The total effective rates were 98.1% and 84.1% respectively (p 1%. Shcherbanovsky and Kapelev (1975) reported the antimicrobial activity of 25 volatile oils from aerial parts and seeds of dill (Anethum graveolens L.) against yeast Saccharomyces vini and Lactobacillus buchneri. Yousef and Tawil (1980) evaluated the bacteriostatic and fungistatic activities of 22 volatile oils, wherein, the cinnamon oil showed the highest activity against the tested bacteria and fungi.
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F. Linalool and chavicol Sweet basil (Ocimum basilicum L.) essential oil has some antimicrobial activity due primarily to the presence of linalool and methyl chavicol (Wan et al., 1998). Lachowicz et al. (1998) evaluated essential oils of sweet basil extracted by distillation against 33 bacteria, yeasts and molds in an agar well assay. The essential oils were active against certain fungi including Mucor and Penicillium species but demonstrated little antimicrobial activity against bacteria in the assay system. A strain of Bacillus cereus and Salmonella Typhimurium were most sensitive to the basil. Addition of 0.1% or 1.0% basil oil to tomato juice medium inactivated 104 CFU/ml of Lactobacillus curvatus (7 days) or Saccharomyces cerevisiae (immediate) at 30˚C, respectively. Wan et al. (1998) did a similar study by screening the essential oil components of sweet basil, linalool and methyl chavicol, against 35 strains of bacteria, yeasts and molds using an agar well diffusion assay. Again, the compounds demonstrated limited activity against most microorganisms except the fungi, Mucor and Penicillium with the well assay system employed. In an system using impedance to monitor growth, 0.125% (v/v) methyl chavicol inhibited Aeromonas hydrophila growth for 48-h at 30˚C while 1% (v/v) of linalool was required. Against Pseudomonas fluorescens, a minimum of 2% (v/v) of the essential oil components were required for inhibition. Methyl chavicol (0.1%) in filter-sterilized fresh lettuce supernatant reduced viable Aeromonas hydrophila by 5-logs and, as a wash for lettuce leaves, the compound was as effective as 125 µg/ml chlorine (Wan et al., 1998). SmithPalmer et al. (1998) reported MICs of basil essential oil of 0.25, 0.25, 0.1, 0.05, and 0.1% for Campylobacter jejuni, E. coli, Salmonella Enteritidis, L. monocytogenes and S. aureus, respectively. Yin and Cheng (1998) detected no antifungal activity against Aspergillus flavus or Aspergillus niger with water extracts of basil or ginger in a paper disk assay. Pattnaik, et al., (1997) tested antimicrobial activity of five aromatic constituents of essential oils (cineole, citral, geraniol, linalool and menthol) against eighteen bacteria (including Gram-positive cocci and rods, and Gram-negative rods) and twelve fungi (three yeast-like and nine filamentous). Linalool was the most effective and inhibited seventeen bacteria, followed by cineole, geraniol (each of which inhibited sixteen bacteria), menthol and citral aromatic compounds, which inhibited fifteen and fourteen bacteria, respectively. Against fungi the citral and geraniol oils were the most effective (inhibiting all twelve fungi), followed by linalool (inhibiting ten fungi), cineole and menthol (each of which inhibited seven fungi) compounds. Lachowicz, et al., (1998) examined essential oils from five varieties of Ocimum basilicum L. plants (anise, bush, cinnamon, dark opal and dried basil) for antimicrobial activity against a wide range of foodborne Gram-positive and Gram-negative bacteria, yeasts and moulds. All five essential oils showed antimicrobial activity against most of the bacteria tested, except Flavimonas oryzihabitans and Pseudomonas species. Synergistic effects were observed between anise oil, low pH (4.2) and salt (5% NaCl). Anise oil demonstrated antimicrobial effect in tomato juice medium and inhibited the growth of Lactobacillus curvatus and Saccharomyces. cerevisiae. G. Vanillin Vanillin (4-hydroxy-3-methoxybenzaldehyde) is a major constituent of vanilla beans, the fruit of an orchid (Vanilla planifola, Vanilla pompona, or Vanilla tahitensis). It has been shown to possess antimicrobial activity (Beuchat & Golden, 1989). Jay and
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Rivers (1984) reported that vanillin was most active as against molds and non-lactic Gram positive bacteria. López-Malo et al. (1995) prepared fruit based agars containing mango, papaya, pineapple, apple and banana with up to 2000 µg/ml vanillin and inoculated each with Aspergillus flavus, A. niger, A. ochraceus, or A. parasiticus. Vanillin at 1500 µg/ml significantly inhibited all strains of Aspergillus in all media. The compound showed least effectiveness in banana and mango agars. Cerrutti and Alzamora (1996) demonstrated complete inhibition of growth for 40 days at 27˚C of Debaryomyces hansenii, Saccharomyces cerevisiae, Zygosaccharomyces bailii and Zygosaccharomyces rouxii in laboratory media and apple puree at aw of 0.99 and 0.95 by 2000 µg/ml vanillin. In contrast, 2000 µg/ml vanillin was not effective against the yeasts in banana puree. These researchers attributed this loss of activity to binding of the phenolic vanillin by protein or lipid in these banana and mango, a phenomenon demonstrated for other antimicrobial phenolic compounds (Rico-Muñoz & Davidson, 1983). López-Malo et al. (1997,1998) studied the effect of vanillin concentration, pH and incubation temperature on Aspergillus flavus, A. niger, A. ochraceus, and A. parasiticus growth on potato dextrose agar. Depending upon species, vanillin in combination with reduced pH had an additive or synergistic effect on growth of the molds. The most sensitive was A. ochraceus (MIC = 500 µg/ml at pH 3.0, ≤ 25˚C or pH 4.0, ≤ 15˚C) and the most resistant was A. niger (MIC = 1000 µg/ml, pH 3.0, 15˚C). Cerrutti et al. (1997) utilized vanillin to produce a shelf-stable strawberry puree. A combination of 3000 µg/ml vanillin, 1000 µg/ml calcium lactate, and 500 µg/ml ascorbic acid preserved strawberry puree acidified with citric acid to pH 3.0 and adjusted to aw 0.95 with sucrose for over 60 days against growth of natural microflora and inoculated yeasts. H. Terpenes Tea-tree oil (an essential oil of the Australian native tree Melaleuca alternifolia) has long been regarded as a useful topical antiseptic agent in Australia and has been shown to have a variety of antimicrobial activities; however, only anecdotal evidence exists for its efficacy in the treatment of various skin conditions. Gustafson et al. (1998) reported on the antimicrobial activity of Australian tea tree (Melaleuca alternifolia) essential oil. The major active components of tea tree oil include terpinen-4-ol, γ-terpinene, αterpinene, α-terpineol, α-pinene, 1,8-cineole and linalool (Gustafson et al., 1998; Hammer et al., 1999b). Against E. coli AG100, the MIC and MBC were 0.25% in microbiological media (Gustafson et al., 1998). Addition of tea tree oil at 0.25% to log and stationary phase cells caused a reduction of > 8 logs of viable E. coli in 30 min and 3-4 logs after 2-h, respectively. Hammer et al. (1999b) determined the antimicrobial effectiveness of tea tree oil and characterized factors affecting its activity. The MICs and MLCs, respectively, determined for the oil against selected bacteria and a yeast were (% v/v): E. coli, 0.12-0.25 and 0.12-0.25, Salmonella Typhimurium, 0.25-0.5 and 0.25-0.5, S. aureus, 0.5 and 0.5-1.0, and Candida albicans, 0.25-0.5 and 0.5. The presence of surfactants, such as Tween 20 or 80, generally increased the MICs against microorganisms, while the presence of minerals or organic matter, such as blood, bovine serum albumin, baker’s yeast, or skim milk, slightly increased or had no effect on the MIC depending upon microorganism. Cox et al. (1998) showed that tea tree essential oil caused leakage and inhibited glucose dependent respiration of E. coli AG100. This indicated a mechanism of action involving disruption of the cytoplasmic membrane.
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Bassett, et al., (1990) conducted a single-blind, randomized clinical trial on 124 patients to evaluate the efficacy and skin tolerance of 5% tea-tree oil gel in the treatment of mild to moderate acne when compared with 5% benzoyl peroxide lotion. The results of this study showed that both 5% tea-tree oil and 5% benzoyl peroxide had a significant effect in ameliorating the patients’ acne by reducing the number of inflamed and noninflamed lesions (open and closed comedones), although the onset of action in the case of tea-tree oil was slower. Aromatic plants from the Labiatae family (Thymus vulgaris, Ocimum gratissimum), the Myrtaceae family (Eugenia caryophyllata, Melaleuca viridiflora) and the Compositae (Helichrysum lavanduloides, H. bracteiferum, H. gymnocephalum, Psiadia altissima) show antimicrobial activity against enteropathogenic and food spoilage organisms (Ramanoelina, et al., 1987). Three oils from Thymus vulgaris, Ocimum gratissimum and Eugenia caryophyllata demonstrated broad-spectrum activity. The essential oil of Melaleuca viridiflora had a high inhibitory effect especially on Gram-positive bacteria. Essential oil from Achillea fragrantissima exerts cidal effect on several Grampositive and Gram-negative bacteria as well as on C. albicans. The active phyto-phenolic compound was identified as terpinen-4-ol (Barel, et al., 1991). Essential oils from Cedronella canariensis (L.) W. et B. inhibit respiratory tract pathogens Bordetella bronchiseptica and Cryptococcus albidus (Lopez-Garcia, et al., 1992). The essential oil from the leaves of Hoslundia opposita contains largely the sesqui-terpenes and sesquiterpene alcohols. These phyto-phenolic compounds show significant activity against Aspergillus niger, Acinetobacter calcoacetica, Brochothrix thermosphacta and Flavobacterium suaveolens. (Gundidza, et al., 1992). Essential oils from Satureja montana L., Rosmarinus officinalis L., Thymus vulgaris L., and Calamintha nepeta (L.) Savi demonstrate potent antimicrobial and fungicide activities (Panizzi, et al., 1993). Camphor and camphene are the major essential oil constituents of Piper angustifolium Lam. These phyto-phenolic compounds are bacteriostatic and fungistatic against Trichophyton mentagrophytes, P. aeruginosa, C. albicans, Cryptococcus neo-formans, Aspergillus flavus, Aspergillus fumigatus, and E. coli (Tirillini, et al., 1996). I. Compounds with limited activity Many herbs and spices have demonstrated limited or no antimicrobial activity. They include anise, bay (laurel), black pepper, cardamom, cayenne (red pepper), celery seed, chili powder, coriander, cumin, curry powder, dill, fenugreek, ginger, juniper oil, mace, marjoram, mint, nutmeg, orris root, paprika, sesame, spearmint, tarragon, and white pepper (Fabian et al., 1939; Webb & Tanner, 1944; Marth, 1966; Zaika & Kissinger, 1979; Tassou et al., 1995). For example, chili, paprika, parsley, red pepper and black pepper at up to 3.0% w/v did not inhibit the growth of L. monocytogenes Scott A at 24˚C (Ting & Deibel, 1992). Hao et al. (1998) showed it (pimento) had little effect on the microorganism in cooked beef. This was suggested to be due to the reduction of activity of the essential oil in the presence of lipids in the food (Hao et al., 1998). Hao et al. (1998) showed that angelica, bay leaf, caraway and marjoram had no activity against L. monocytogenes in cooked beef. Tassou et al. (1995) evaluated the effect of mint (Mentha piperita) essential oil on Salmonella Entertidis and L. monocytogenes in culture medium and three foods. The effect of the essential oil was variable and depended on pH, temperature and the food. Eucalyptus, marjoram and peppermint were inhibitory primarily to the Gram-positive
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bacteria. Bay (laurel) was found by these researchers to have inhibitory and bactericidal activity in the ranges of 0.002-0.075% and 0.04-0.5%, respectively, against the five bacteria. This is in agreement with some reports (Hammer et al., 1999a) and in contrast to other reports that bay has little or no activity (Karapinar & Aktug, 1986; Hao et al., 1998). Perhaps the most unique finding by Smith-Palmer et al. (1998) was that nutmeg essential oil was inhibitory to L. monocytogenes at < 0.01% and bactericidal at 0.05% at 35˚C. The activity of nutmeg was highly dependent upon temperature as the MIC and MBC increased to 0.5% and > 1% at 4˚C. The antimicrobial effectiveness of bay, cinnamon and thyme was not influenced by a temperature shift from 35 to 4˚C. Huhtanen (1980) showed that 10% ethanol extracts of selected spices were inhibitory to Clostridium botulinum including (MIC in µg/ml in parenthesis): mace (31), bay (125), black pepper (125), nutmeg (125), and white pepper (125). Ejechi et al. (1998) found that high concentrations (15-20% v/v) of water extracts of ginger and nutmeg could inhibit the growth of natural spoilage microflora of mango juice for 1 month at 30˚C. This high concentration of extract was not acceptable on a sensory basis. However, 4% of each extract combined with heating the mango juice to 55˚C prevented growth of both yeast and mold in the juice and produced a product with satisfactory sensory attributes. Kubo et al. (1991) determined the antimicrobial activity of cardamom essential oil and 10 components of the nhexane extract of cardamom using a broth dilution assay. Against food-related bacteria, eugenol (also present in cloves) was most effective against the Gram-positive bacteria Bacillus subtilis and S. aureus (MIC 400-800 µg/ml) while, with the exception of E. coli which was inhibited by 400 µg/ml eugenol, none of the components was inhibitory to the other Gram-negative bacteria, Pseudomonas aeruginosa or Enterobacter aerogenes. The most effective antimicrobial components against fungi were geraniol, limonene and α-terpinene. Cardamom essential oil was very limited in its antimicrobial activity generally requiring 800 to > 1,600 µg/ml to inhibit food-related bacteria and fungi (Kubo et al., 1991). Turmeric was shown to inhibit a variety of bacteria, including B.cereus, S. aureus, E. coli, and Lactobacillus plantarum (Bhavani Shankar & Sreenivasa Murthy, 1979). Whereas, nutmeg, curry powder, mustard, black pepper, and sassafras could moderately inhibit V. parahaemolyticus (Beuchat, 1976). The spice, Aframomum danielli, on a wet weight basis with a moisture content of 10.5%, protein content of 8.2% (dry matter basis) could inhibit the growth of Salmonella enteriditis, Pseudomonas fragi, P. fluorescens, Proteus vulgaris, Streptococcus pyogenes, S. aureus, Aspergillus flavus, A. parasiticus, A. ochraceus and A. niger. The MIC for Klebsiella pneumoniae and P. aeruginosa was 1 in 32 whilst the MIC for S. aureus was 1 in 8,000 (Adegoke & Skura, 1994). J. Mechanisms of action Some studies have focused on the mechanism by which spices or their essential oils inhibit microorganisms. Since it has been concluded that the terpenes in essential oils of spices are the primary antimicrobials, the mechanism most likely involves these compounds. Many of the most active terpenes, e.g., eugenol, thymol and carvacrol, are phenolic in nature. Therefore, it would seem reasonable that their modes of action might be related to other phenolic compounds. The mode of action of phenolic compounds is generally thought to involve interference with functions of the cytoplasmic membrane including proton motive force and active transport (Eklund, 1985; Davidson, 1993). In fact, Juven et al. (1994) hypothesized that inhibition by thymol of Salmonella Typhimurium
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was due to a reaction of the compound with proteins in the cytoplasmic membrane of the microorganism. This caused changes in permeability of the membrane resulting in possible leakage and affected the proton motive force. In addition, terpenes may have other antimicrobial mechanisms. Conner and Beuchat (1984) suggested that spice essential oils may inhibit enzyme systems in yeasts, including those involved in energy production and synthesis of structural components. Conner et al. (1984) demonstrated energy depletion in yeasts caused by essential oils of several spices including clove, thyme, oregano and cinnamon. In addition, ethanol production, respiratory activity and sporulation of yeast cells was also influenced by these essential oils.
IV. SUMMARY Spices and herbs and their essential oils have varying degrees of biological activity. Of the 70 herbs and spices officially recognized as useful for food ingredients (Lindsay, 1996), only a handful have demonstrated significant antimicrobial activity. In many cases, concentrations of the antimicrobial compounds in herbs and spices are too low to be used effectively without adverse effects on the sensory characteristics of a food. However, they may contribute to the overall ‘hurdle’ system present naturally in a food product. The most consistent antimicrobial activity among herbs and spices has been found with components of cloves, cinnamon, mustard seed, oregano, rosemary, sage, thyme, and vanillin. Effective phyto-phenolic agents preserve food by various mechanisms including stasis (growth inhibition of microorganisms) and cidal (direct destruction of microorganisms) effects. Certain phyto-phenolic agents such as from olive oil seem to deliver multifunctional physiological benefits to the consumer, therefore are highly attractive to the health food industry. Since phyto-phenolic compounds have been in the food supply and consumed for many years, these natural phytochemicals appear to be safe when compared to new synthetic preservatives.
V. REFERENCES 1. 2.
3. 4. 5. 6. 7.
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Adegoke, G.O., and Skura, B.J. 1994. Nutritional profile and antimicrobial spectrum of the spice Aframomum danielli K. Schum. Plant Foods Hum. Nutr. 45:175-182. Aeschbach, R., Loliger, J., Scott, B.C., Murcia, A., Butler, J., Halliwell, B., and Aruoma, O.I. 1994. Antioxidant actions of thymol, carvacrol, 6-gingerol, zingerone and hydroxytyrosol. Food Chem. Toxicol. 32:31-36 Akgul, A., and Kivanc, M. 1988. Inhibitory effects of selected Turkish spices and oregano components on some foodborne fungi. Int. J. Food Microbiol. 6:263-268. Ali-Shtayeh, M.S., Al-Nuri, M.A., Yaghmour, R.M., and Faidi, Y.R. 1997. Antimicrobial activity of Micromeria nervosa from the Palestinian area. J. Ethnopharmacol. 58:143-147. Al-Khayat, M.A., and Blank, G. 1985. Phenolic spice components sporostatic to Bacillus subtilis. J. Food Sci. 50:971-974. Al-Meshal, I.A. 1986. Isolation, and characterization of a bioactive volatile oil from Ducrosia ismaelis Asch. Res. Commun. Chem. Pathol. Pharmacol. 54:129-132. Amaya Guerra, C.A., Othon Serna Saldivar, S.R., Cardenas, E., and Nevero Muunoz, J.A. 1997. Evaluation of different solvent systems for the extraction and fractionation of oleoresins from guajillo peppers. Arch. Latinoam. Nutr. 47:127-130. Avato, P., Vitali, C., Mongelii, P., and Tava, A. 1997. Antimicrobial activity of polyacetylenes from Bellispernnis and their synthetic derivatives. Planta Med. 63:503-507.
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9. 10. 11. 12. 13. 14. 15. 16.
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I. INTRODUCTION Saponins are a group of naturally occurring glycosides which are predominantly found in the plant kingdom, however, certain lower marine animals also contain these compounds. They can be found in different plant parts including roots, shoots, flowers and seeds. The common feature of most of the saponins is the formation of soapy lather when shaken in water solution. The height of the froth and the time of its disappearance have been often used as a semiquantitative test for characterization of plant species with respect to saponin content. Most literature concerning saponin distribution is based on this test. In the Orient, saponins were used in traditional folk medicine or as a soap and thus, in many cases trivial names of saponin-rich plant species are derived from this feature e.g. soapwort (Saponaria officinalis), soaproot (Chlorogalum pomeridianum), soapbark (Quillaja saponaria), soapberry (Sapindus saponaria), soapnut (Sapindus mukurossi) (Hostettmann & Marston, 1995). Depending on the structure saponins may show hemolytic, antimicrobial, membrane depolarizing, cholesterol binding and allelopathic activities. Hemolytic activity of saponins in vitro was reported by Kobert as early as 1887 and was based on the destruction of erythrocyte membranes (lysis) and release of hemoglobin. From the nutritional point of view hemolytic activity does not seem to create any problems as saponins neither cross membrane barrier nor enter the blood stream. This characteristic was applied in a number of hemolytic semiquantitative tests for saponin determination and has been reviewed by Birk (1969). Cholesterol binding and permeation of the epithelial barrier may have nutritional consequences and much work has been recently devoted to these effects (Gee et al., 1998; Malinow et al., 1978, 1981). These aspects generated dramatic progress in the development of isolation, structure determination and testing techniques of individual saponins. Antimicrobial activities are important to the plant for protection against pathogens. The localization of saponins with higher antimicrobial activity in plant parts previously exposed to pathogens suggests such a function. Aerial parts of some plants may
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cumulate bitter taste saponins, a feature important in plant protection against herbivores (Oleszek et al., 1999).
II. OCCURRENCE Saponins are widely distributed in plant species, about 100 families. As reported by Gubanov et al. (1970) 76% of Asian plant families contain saponins. They are found in edible plants such as soya, beans, peas, oat, Solanum and Allium species, tomato, asparagus, tea, peanut, spinach, sugar beet, yam and blackberry; in plants used as animal feed such as alfalfa, clover, legumes, forage and cover crops, sunflower, horse chestnut, guar and lupine; and in plants used as flavorings, health foods, tonics etc. including fenugreek, liquorice, nutmeg, Quillaya, Yucca, Gypsophila, herbs, edible seeds, health foods, and ginseng (Price et al., 1987). Their concentration in plants ranges from traces up to 10% of dry matter as in the Yucca schidigera trunk. The concentration depends on the cultivar, age, physiological stage and geographical location of the plant. Considerable qualitative and quantitative variation also exists between plant parts. For example alfalfa seeds contain only low toxicity soyasapogenol glycosides (0.2% of DM), while during germination glycosides of medicagenic acid, zanhic acid and hederagenin are synthesized (Oleszek, 1998). Roots of alfalfa contain medicagenic acid, zanhic acid, hederagenin and soyasapogenol glycosides with a total concentration of saponins 2.5% DM while aerial parts possess similar glycosides but at lower concentration 0.1- 1.5% DM (Nowacka & Oleszek, 1994). Depending on the origin of the variety in a saponin mixture, soyasapogenol glycosides, medicagenic acid glycosides or zanhic acid tridesmoside may dominate. As mentioned above the presence of saponins in plant extract can be simply demonstrated by the froth formation after shaking in water solution. Nevertheless, some saponins, especially those with two or three branched sugar chains do not form stable froth. On the other hand, certain plant extracts not containing saponins may also produce froth, and may mislead. Some saponins show hemolytic activity and this feature in some cases could be used as a semiquantitative test, with several modifications (Birk, 1969). In general, saponin-containing material or its water extract is mixed with ox blood or with washed erythrocytes in isotonic buffered solution (0.9% NaCl). After 20-24 h incubation, samples are centrifuged and hemolysis is indicated by the presence of hemoglobin in the supernatant. According to the European Pharmacopoeia, a unit hemolytic index (HI) is defined as the amount (in milliliters) of ox blood (2%, v/v) hemolyzed by 1-g of crude saponins or plant material. The saponin mixture of Gypsophila paniculata L. (HI = 30 000) or Saponin white (Merck, HI = 15 000) are usually used as reference. Hemolytic indices of saponins are calculated according to the following equation: HI = HIstd x a/b; where HIstd is the hemolytic index of standard saponin, and a and b are the means of lowest concentration from each replicate of standard and saponins, respectively, at which full hemolysis occurred. Mackie et al. (1977) measured the absorbance at 545 nm of the supernatant after hemolysis and defined one unit of activity as the quantity of hemolytic material that caused 50% hemolysis. The other modification of the above method is a hemolytic micromethod. In this assay, bovine blood is stabilized with sodium citrate (3.65% w/v) and mixed with gelatin solution. Gelatin (4.5 g) is dissolved in 100 ml of isotonic buffered solution and 75 ml of
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FIGURE 1. Hemolytic test performed on blood-gelatin covered plates. Black spots – mashed alfalfa plant material; transparent rings – hemolytic zones; background in original – red.
this solution is mixed with 20 ml of the blood. Gelatin/blood mixture is spread on a glass plate (10 x 20 cm) to a thickness of 0.5 mm. After coagulation, plates are used for hemolytic tests. Saponin samples (10 ml) or mashed fresh plant material is placed in localized areas on the gelatin/blood-covered plates and after 20 h the width of the resulting hemolytic rings are measured (FIGURE 1). Standard saponin is measured as a reference control on each plate. Detailed descriptions of HI and microhemolytic methods are described by Oleszek (1988). Saponins can also be quantified in bio-assays using organisms such as Trichoderma viride (Zimmer et al., 1967), Tribolium castaneum (Shany et al., 1970), lettuce seed germination (Pedersen et al., 1967) or with gravimetry (van Atta et al., 1961), spectrophotometry (Hiai, 1976; Baccou, 1977; Gestetner, 1966) and chromatography (TLC, GC, HPLC) (Besso et al., 1979; Domon et al., 1984; Kitagawa et al., 1984; Slacanin et al., 1988; Oleszek et al., 1990; Tava et al., 1993; Xin et al., 1994). Qualitative assay for saponins can be performed with TLC on silica gel or reversed phase C18 plates. Most often used solvents for silica gel TLC include chloroform-methanol-water (7:3:1; 65:35:10 and similar combinations), ethyl acetate-acetic acid-water (7:2:2), n-butanol-ethanol-ammonia (7:2:5), n-butanol-acetic acid-water (BAW 4:1:5, upper layer), chloroform-methanol-acetic acid-water (60:32:12:8), n-butanol saturated with water, n-butanol-ethyl acetate-water (100:25:50), ethyl acetate-pyridinewater (30:10:30, upper phase, for glycoalkaloids). For reversed phase (C18, C8) plates almost exclusively different proportion of water-methanol and water-acetonitrile are used depending on the polarity of analyzed saponins. Several sprayers are used for visualization of saponins and depending on the structure, they may produce different colored spots. The most common sprayers are vanillin-sulfuric acid (a 1% solution of vanillin in ethanol, mixed with 3% solution of perchloric acid in water in a 1:1 ratio and sprayed onto the TLC plate followed by the 10% solution of sulfuric acid in ethanol); Liebermann-Burchard (methanol:acetic anhydrate:sulfuric acid, 50:5:5 v/v) and Ehrlich reagent (1 g p-dimethylaminobenzaldehyde in 50 ml 36% HCl mixed with 50 ml ethanol). All listed sprayers require heating of the plates for several minutes at 105-120˚C. The vanillin-sulfuric acid reagent generates color product with most of the saponin aglycones but the reac-
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tion is not very specific and certain other classes of substances may also react. Liebermann-Burchard reagent produces color spots with aglycones (blue, green, pink, brown, yellow) and with glycosides e.g. green for medicagenic acid, pink for hederagenin, bricky for soyasapogenol, yellowish for zanhic acid, brown for steroidal furostanol and spirostanol saponins. The Ehrlich reagent is highly specific for furostanol steroidal saponins and produces pink-red spots, while spirostanol glycosides are not visualized. This reagent could effectively distinguish these two groups of compounds. Many of listed sprayers are successfully used for spectrophotometric determination of saponins. This has, however, to be performed with caution, since certain compounds present in the sample matrices cause interference. Gas chromatography has been used for determination of aglycones liberated after hydrolysis of saponins. This technique has been used for determination of trimethylsilyl ethers of soyasapogenols and medicagenic acid (Jurzysta & Jurzysta, 1978) trimethylsilyl ethers of soyasapogenol A and B in soybean (Kitagawa et al., 1984), dimethyl ester, di(trimethylsilyl)ether of medicagenic acid (Brawn et al., 1981), methylated-acetylated medicagenic acid, hederagenin and soyasapogenols B, C, D, E and F (Tava et al., 1993), trimethylsilyl ethers of panaxadiol and panaxatriol from ginseng (Sakamoto et al., 1975) and methyl ester TMS ether of glycyrrhetinic acid from Glycyrrhiza radix and human serum (Bombardelli et al., 1976, 1979; Itoh et al., 1985). Formation of artifacts during saponin hydrolysis and artifact formation during derivatization and analysis is a limitation to this technique. Derivatized compounds are often poorly separated by this method. High performance liquid chromatography (HPLC) seems to be the most reliable technique for quantification. The main problem in chromatographic determination is the lack of chromophores in saponin molecules, which creates a problem for UV detection. The non-specific detection at 200-210 nm is possible, however, this requires a careful precolumn purification of extracts, and removal of other components from the matrix (Domon et al., 1984). Pre-column derivatization of saponins with reagents introducing chromophores is an alternative (Besso et al., 1979; Slacanin et al., 1988).
III. MOLECULAR PROPERTIES Saponins consist of non-sugar aglycone coupled to sugar chain units. These sugars could be attached to the aglycone either as one, two or three side chains, and the terms monodesmoside, bidesmoside and tridesmoside has been given to these saponins, respectively (Greek desmos = chain) (Wulf 1968). According to the nature of aglycone they could be divided into the groups of saponins containing steroidal or triterpene (FIGURE 2) aglycones - sapogenins. Some authors also include steroidal glycoalkaloids of solanidans and spirosolan class in the group of saponins (FIGURE 3). Steroidal skeletons have in most cases furostanol or spirostanol form; furostanol glycosides usually have a bidesmosidic and spirostanol monodesmosidic nature. Both steroidal and triterpene saponins may have a number of functional groups (-OH, -COOH, -CH3) causing great natural diversity only because of aglycone structure. Over 100 steroidal and probably an even higher number of triterpene saponins have been known (Hostettmann & Marston, 1995). This diversity could be further multiplied by the composition of sugar chains, their number, branching patterns and substitution. It is well known that even within one plant species, distinct parts may harbor structurally different saponins. This diversity makes isolation and identification of single saponins quite difficult.
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STEROIDAL GROUP
TRITERPENE GROUP
Cholestan
ß - Amyrin type (oleananes)
Spirostan
α - Amyrin type (ursanes)
Furostan
Lupeol type (lupanes)
FIGURE 2. Sapogenin skeletons – Steroidal and Triterpene
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GLYCOALKALOIDS GROUP
Solanidan
Spirosolan
FIGURE 3. Sapogenin skeletons – Glycoalkaloids
Early work on saponins included hot extraction with aqueous methanol or ethanol of defatted plant material, followed by evaporation of alcohol and extraction of saponins into n-butanol (Wall et al., 1952). In this liquid-liquid extraction, highly polar components present in extract matrix e.g. saccharides stay in the water solution giving some purification of the extract. However, in most of the cases evaporation of butanol produces dark-brown solid rich solution with many interfering compounds. Some authors propose dialysis for removal of small water-soluble molecules (Massiot et al., 1988). The next step of purification may include precipitation of saponins from water solution with lead acetate, barium hydroxide or cholesterol or precipitation from alcohol solution with diethyl ether or acetone. Such treatments produce crude saponin mixtures. Nevertheless, these procedures also have many disadvantages and some, such as cholesterol precipitation, are inconvenient due to difficulties in ensuring the complete washing of non-precipitated saponin from the viscous precipitate. The extraction with hot aqueous methanol may lead to the formation of -OCH3 derivatives, lactones, both in triterpene and steroidal saponins or may result in the degradation of genuine saponins into their artifacts as in the case of soybean saponins (Massiot et al., 1996). Such transformations occur on the aglycone skeleton or on the sugar part, or consist in the loss of labile substituents. In liquidliquid extraction, some highly polar saponins (bidesmosides and tridesmosides) could be lost or extraction may not be quantitative. This has been observed in zanhic acid tridesmoside present in alfalfa aerial parts (Oleszek et al., 1992). In the Wall’s procedure, tridesmoside, in spite of its very high concentration in some cultivars, remained in water with carbohydrates. The alternative for Wall’s procedure is solid-phase extraction (SPE) on reversed phase (C8, C18) sorbent (Oleszek, 1988). In the SPE method, saponin extract (aqueous 10-20% methanol) can be loaded on a short column and then washed with methanolwater. Depending on the concentration of methanol different classes of matrix components can be removed. The water can easily remove all carbohydrates while watermethanol mixtures (up to 40% of methanol) may remove phenolics, including most of the flavonoids. Saponins can be washed out with solvents containing more than 40% methanol; depending on the concentration selective extraction of different classes of saponins can be achieved. This, however, requires preliminary tests for different classes of saponin extract that can be performed on ready to use 1-2 cm3 cartridges. Selectivity of the C18 sorbent to retain saponins strongly depends on the pH of the loaded sample, which is especially convenient in separation of saponins having COOH groups. The SPE © 2000 by CRC Press LLC
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FIGURE 4. TLC chromatogram of alfalfa root saponins; s – crude saponin mixture; 1-25 individual saponins.
method is especially convenient with steroidal saponins. In many cases, this is a good procedure for separation of highly purified crude saponin mixtures for evaluation of biological activity. The separation of crude mixtures into individual saponins is quite a challenge. The wide range of polarities of individual glycosides makes it almost impossible to separate individual saponins in one run. Open column or low-pressure liquid chromatography on silica gel and reversed phase sorbents has to be applied in combination. The first separation usually provides saponin fractions that consist of several glycosides with similar retention properties. For further separation, it is necessary to switch to another sorbent or solvent system. In the case of triterpene alfalfa saponins, separation on C18 sorbent in water-methanol gradient is very convenient and further purification of individual saponins can be accomplished on silica gel columns (Oleszek et al., 1990). However, initial separation on silica gel column with n-butanol saturated with water followed by C18 column also yields good separation (FIGURE 4) (Bialy 1998). For steroidal saponins, best separations can be achieved by silica gel column chromatography washed with chloroformmethanol mixtures followed by C18 separation with methanol-water mixtures.
IV. ANTIMICROBIAL ACTIVITY A. Antibacterial activity The general principle of the action of saponins on microorganism is their interaction with membrane sterols. Thus, the bacteria should not be sensitive to saponins, as their membranes are low in cholesterol. However, recent report on the saponin-sensitive and insensitive Trichoderma viride strains indicate that fatty acid composition of membranes may equally be important in this respect (Gruiz, 1966). Thus, a number of saponins, both triterpene and steroidal, show antibacterial activities (TABLE 1). Antibacterial activity of saponins has been extensively reviewed by Takeya (1997) and Tamura (1996).
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The degree of activity depends on the saponin structure, target microorganism and may range from 5 ppm as reported for gitogenin glycoside (I) (Masamitsu et al., 1995) up to 5-10 mg/ml found for saponins from common ivy (hederagenin glycosides) (Cioaca et al., 1978). In general, the common ivy saponins were more active against Gram-positive than Gram-negative bacteria with minimal inhibitory concentrations (MIC) of 0.31.25 and 1.25-5 mg/ml, respectively. Positive reactions between antibiotics (ampicillin, kanamycin, cephalexin, oxytetracycline and chloramphenicol) and ginseng saponins were studied by checkerboard method (Kim et al., 1987). It was documented that ampicillin, kanamycin, oxytetracycline and chloramphenicol against Bacillus subtilis and ampicillin and cephalexin against Staphylococcus aureus were synergistic with ginseng saponin. No antagonism between saponins and antibiotics could be observed. Quillaya saponins show emulsifying properties enhancing the antibacterial effectivity of fumaric acid in food preservation. Antibacterial agent was prepared by mixing 100 g of fumaric acid and 0.5 g Quillaya saponin powder (Nishina et al., 1992). Mixing saponins with acetic acid was shown to be an effective antimicrobial composition for the control of bacteria grown on the skin after perspiration (Tatebe, 1986). The major effect of saponins on bacteria is the leakage of protein and certain enzymes from their cells (Zablotowicz et al., 1996, Hoagland et al., 1996). The ß-aescin, glycyrrhetic acid and medicagenic glycosides increased extracellular protein leakage from three bacterial strains including Pseudomonas fluorescens RA-2, Curtobacterium flaccumfaciens JM-1011 and Bacillus thuringiensis UZ404, as measured 24 h after treatment with 500 µM saponin solutions. Betulin and hecogenin had no influence or slightly reduced protein leakage, while soyasaponin I increased leakage in case of C. flaccumfaciens and reduced it by 20 and 50% in P. fluorescens and B. thuringiensis, respectively. Different effects of structurally divergent alfalfa saponins were also observed on enzymatic activity, FDA-esterase and TTC-dehydrogenase in the B. thuringiensis but not in P. fluorescens (Oleszek et al., 1999). These data clearly indicate that bacterial membranes can be affected by certain saponins, resulting in a significant loss of vital activity, especially in some Gram-positive genera such as the Bacillus sp. B. Antifungal activity Among the saponins, those with triterpene and spirostanol skeleton generally demonstrate antifungal activities (TABLE 2). Furostanol saponin with bisdesmosidic nature lack bacteriostatic and fungicidal effects, and does not complex with cholesterol. Complexing with membrane sterols, proteins and phospholipids seems to be a major mechanism that predispose sensitivity of a microbe to saponins, but the effect is relatively nonspecific. In the case of fungi, as shown by Gruiz (1996), ergosterol content of saponin sensitive and insensitive Trichoderma viride strains did not differ significantly. In both cases, however, endogenous saponin treatment significantly increased ergosterol level. Considerable changes after saponin treatment were noticed in the lipid composition of sensitive and insensitive strains. It was concluded that metabolic changes in fatty acid composition of membrane phospholipids discriminate fungus sensitivity to exogenous saponins. Regarding the structural features of saponin, their fungicidal activities are determined by the aglycone structure and also by the number, quality and branching patterns of sugar substitution. The aglycone by itself may show very high antifungal activity. Medicagenic acid (FIGURE 5) in a free form may totally inhibit T. viride at the concentra-
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TABLE 1. Antimicrobial acitivity of saponins from different plant sources Plant source
Saponin
Microorganism
MIC
Reference
Aesculus hippocastanum
triterpene
Agrobacterium tumefaciens Rhizobium meliloti Bradyrhizobium japonicum Pseudomonas fluorescens Several species Streptococcus mutans Saccharomyces cerevisiae Bacillus cereus, B. subtilis 22 different bacteria Bacillus subtilis M45 Staphylococcus aureus Debaryomyces polymorphus Zygosaccharomyces rouxii Agrobacterium tumefaciens Corynebacterium insidiosum Pseudomonas lachrymans Coryno. michiganense Xanthomonas campestris Staphylococcus aureus Pseudomonas aeruginosa C. diphtheriae Pseudomonas aeruginosa Bacillus subtilis Cryptococcus neoformans Cryptococcus neoformans 8 bacterial strains Streptococcus spp. Escherichia coli Bacillus anthracis Staphylococcus aureus Klebsiella pneumoniae Salmonella typhi Staphylococcus aureus Streptococcus faecalis Escherichia coli
100 µM 100 µM 100 µM 25 µM modest 10 µg/ml
Oleszek et al., 1999
Astragalus melanophrurius triterpene Beta vulgaris triterpene Capsicum annum steroidal Hedera helix Hedyotis molicaulis Henricia laeviuscola Hosta sieboldiana
triterpene triterpene steroidal steroidal
Medicago sativa
triterpene
Medicago sativa
triterpene
Sanicula europaea Sapindus saponaria
triterpene triterpene
Smilax aspera Solenostemma argel
steroidal steroidal unspec.
Symphytum officinale
triterpene
10 ppm 5 ppm
Calis et al., 1997 Sasazuka et al., 1995 Gal, 1968 Cioaca et al., 1978 Masataka et al.,1998 Andersson et al., 1989 Masamitsu et al., 1997 Timbekova et al., 1996
Boguslavsky et al, 1992 Przyborowski et al., 1967 Lemos et al., 1992
Petritic et al., 1969 Bruno 1968 El Hady et al., 1994
20 µg/ml
Ahmad et al., 1993
tion as low as 2.2 µg/ml, but the activity of hederagenin differing slightly in the structure from medicagenic acid, has been reduced, while soyasapogenol B structurally related to these two sapogenins is lacking in any activity. In the case of medicagenic acid, the maximum activity has been found when all functional groups (-COOH, -OH) were free. Blockage of the two carboxylic groups led to the impaired growth, so that 50-60% of the growth was maintained even at a concentration of 100 µg/ml. Also blocking of the -OH groups in the aglycone produced a very significant lowering of antifungal activity (Oleszek et al., 1988). Glycoalkaloid saponin, α-tomatine owes also its antimicrobial effect to the tomatidine moiety (Arneson & Durbin, 1968, Jadhav et al., 1981) and sugar beet saponins to oleanolic acid (Sasazuka et al., 1995). It is suggested that glycosides are ineffective against microorganisms. However, aglycones released from them by the enzymes present on the cell surface are antimicrobial. In some in vitro tests, the aglycones could elicit marginal activity, and this may happen due to their poor water solubility, as sapogenins are usually hydrophobic compounds. This problem could be circumvented by
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Fungal species
steroidal
Albizzia lebbek Allium ampeloprasum Allium sativum Asparagus officinalis Asparagus officinalis
unspec. steroidal steroidal steroidal steroidal
Asparagus officinalis Avena sativa Avena sativa
steroidal triterpene triterpene
Bellis perennis
triterpene
Camellia japonica
triterpene
Camellia japonica Camellia oleifera
triterpene triterpene
Camelia spp. Celmisia petriei Chisocheton paniculatus
triterpene triterpene steroidal
Clerodendrum wildii Dolichos kilimandscharicus Dracaena mannii
triterpene triterpene steroidal
Aspergillus spp., C. albicans, Rodotorula glutinis, S.cerevisiae Macrophomina phaseolina Mortierella ramanniana Candida albicans Trichophyton rubrum, C. albicans Cryptococcus spp., Trichophyton spp. Microsporum spp., Epidermophyton spp. Several fungi Fusarium avenaceum Botritis cinerea, Fusarium lini Altenaria spp. Candida spp., Microsporum spp. Trichophyton spp., Aspergillus niger Botritis cinerea, Cochliobolus miyabeanus Pyricularia oryzae, Pestalotia longiseta T. mentagrophytes, Epidermophyton floccosum Trichopyton spp., Epidermophyton flocosum Microsporum audouinii Pilicularia oryzae, Cochliobolus miyabeanus Cladosporium cladosporoides Curvularia verruciformis, Altenaria solani Dreschleva oryzae Cladosporium cucumerinum Cladosporium cucumerinum Trichophyton spp., Cladosporium carrionii Trichosporon cutaneum, Geotrichum candidum Microsporum spp., Phialophora verrucosa Ramichloridium subulatum, Exophiala jeanselmei
© 2000 by CRC Press LLC
MIC
Reference Page 10
Saponin
Agave sisalana
Uikawa & Purchio, 1989 32.8 µg/ml 10 µg/disc 100 µg/ml 2-3 µg/ml 0.5-8 µg/ml
Ahmad et al., 1990 Sata et al., 1998 Matsura et al., 1996 Magota et al., 1994 Shimoyamada et al., 1990
2.5 mg/ml
Shimoyamada et al., 1996 Luening et al., 1978 Singh et al., 1992 Willigmann et al., 1992 Nagata et al., 1985
25 µg/ml 0.1-3 µg/ml 10 µg/ml
Uemura et al., 1997 Jin et al., 1993 Hamaya et al., 1984 Rowan & Newman, 1984 Bordoloi et al., 1993
3.3 µg/plate 2-5 µg/plate 6-12.5 µg/ml 6.25 µg/ml 12-50 µg/ml 25 µg/ml
Toyota et al., 1990 Hostettmann et al., 1996 Okunji et al., 1990, 1996
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TABLE 2. Antifungal acitivity of saponins from different plant sources
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Medicago sativa
triterpene
Medicago sativa Medicago sativa Medicago sativa Medicago spp. Mollugo pentaphylla Nicotiana tabacum Pisum sativum Polemonium caeruleum Polygala vulgaris Primula acaulis Rapanea melanophloeos Rudgea viburnioides Ruscus aculeatus Sapindus mukurossi Serjania salzmanniana
triterpene triterpene triterpene triterpene triterpene steroidal triterpene triterpene triterpene triterpene triterpene triterpene steroidal steroidal triterpene
(Contd.) © 2000 by CRC Press LLC
10mM 150 µg/ml 10-50 µg/ml 17-50 µg/ml 3.5-7 µg/ml 50 µg/ml 7-25 µg/ml 5-10 µg/ml 17-50 µg/ml
1.5 µg/plate 150-300 µg/ml
1 µg/plate
1.5 µg/plate 8-16 µg/ml
Favel et al., 1994 Bader & Hiller, 1995 Bader & Hiller, 1995 Jadhav et al., 1981 Osbourn et al., 1995 Melton et al., 1998 Schlosser, 1976 Phongpaichit et al., 1995 Xie et al., 1998 Oleszek et al., 1988 Martyniuk et al., 1996 Zehavi et al., 1993 Zehavi et al., 1996 Oleszek, 1996 Boguslavsky et al., 1992 Zentmeyer & Thompson,1967 Jurzysta & Waller, 1996 Hamburger et al., 1989 Grunweller et al., 1990 Christian et al., 1989 Hiller et al., 1981 Chesne et al., 1983 Margineau et al., 1976 Ohtani et al., 1993 Young et al., 1998 Guerin & Reveillere, 1984 Tamura et al., 1990 Ekabo et al., 1996
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triterpene triterpene triterpene steroidal steroidal steroidal steroidal triterpene unsp. triterpene triterpene triterpene
Bar-Nun & Mayer, 1990 Timon-David et al., 1980
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Hedera helix Heteropappus altaicus Heteropappus biennis Lycopersicon esculentum Lycopersicon esculentum Lycopersicon esculentum Lycopersicon esculentum Maesa ramentacea Malus meliana Medicago lupulina Medicago sativa Medicago sativa
100 mg/kg 0.5 mg/ml
305
triterpene triterpene
25 µg/ml 100 µg/ml
Saponins
Echallium elaterium Hedera helix
C.albicans, Rhodotorula sp., Fonsecaes pedrosoi, Candida tropicalis Botritis cinerea Candida albicans CS60 Microsporum canis Candida glabrata Candida spp. Candida spp. Aspergillus spp., C. albicans, Trichophyton spp. Gaeumannomyces graminis Septoria lycopersici, Cladosporium fulvum Corticium rolfsii 10 fungal species Food preservation Trichoderma viride Gaeumannomyces graminis Sclerotium rolfsii, Rhizoctonia solani, A. niger Fusarium oxysporum, Cephalosporium gramineum T. mentagrophytes, Epidermophyton floccosum Microsporum canis, Cryptococcus sp., C.albicans Trichoderma viride Trichoderma viride, Candida albicans Phytophthora cinnamomi Trichoderma viride Cladosporium cucumerinum Cladosporium cucumerinum, Puccinia recondita Fusarium solani yeasts, dermatophytes, molds Ceratocystis ulmi Candida spp. Cladosporium cucumerinum Cladosporium cladosporioides Aspergillus fumigatus, T. mentagrophytes Cladosporium cucumerinum Cryptococcus neoformans, Candida albicans
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Fungal species
MIC
Reference
Silphium perfoliatum Solanum tuberosum
triterpene steroidal
10-1000 µg/ml
Davidyants et al., 1997 Jadhav et al., 1981
Solenostemma argel
unspec.
Solidago virgaurea Trigonella foenum-graecum
triterpene steroidal
Trillium glandiflorum
steroidal
Yucca schidigera
steroidal
Zygophyllum spp.
triterpene
Drechslera graminea, R. nodosus, R. nigricans Trichoderma viride, Cladosporium fulvum Helmintosporium carbonum, Fusarium caeruleum Asperillus, Penicillim, Chrisoporium, Candida spp C. neoformans, Mucor, Rhodotorula Candida spp. Rosellinia necatrix, T. harzianum, T. viride Candida albicans C. albicans, S. cerevisiae, T. mentagrophytes Cryptococcus neoforman, Aspergillus spp Saccharomyces spp., Candida albicans C. farmata, Hansenula spp., Cryptococcus spp. Pichia spp., Debaromyces spp., Trichophyton spp. Zygosaccharomyces spp., Sabouraudites canis Epidermophyton floccosum Verticillium albo-atrum, Fusarium oxysporum
El Hady et al., 1994
200 µg/ml 50-100 µg/ml 1.5-12.5µg/ml 31-62 µg/ml 31.3 µg/ml 31.3 µg/ml 31.3 µg/ml 31.3 µg/ml
Bader and Hiller, 1995 Sauvaire et al., 1996 Hufford et al., 1988 Tanaka et al., 1996
Oui et al., 1994
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medicagenic acid
soyasaponin I: R1= CH2OH R2=Rha soyasaponin II: R1= H R2=Rha
glycyrrhizin: R=GlcA-GlcA
diosgenin (25R) digitogenin
FIGURE 5. Structures of selected saponins and sapogenins with extensively elucidated biological activities.
the incorporation of the aglycone to cyclodextrin (CD) (Sasazuka et al., 1995). The antimicrobial activity of oleanolic acid (OA) incorporated into CD was similar to that of OA. The solubility of ß-CD was 1.85 g/100g of water at 25˚C, while that of OA-ß-CD was 3.85 g/100 g of water and increased with the temperature. Structurally divergent glycosides of the same aglycone molecule may show a wide range of activities. In this respect, monoglycosides with one sugar attached demonstrate similar activity to the aglycone. This was proven with medicagenic acid glucoside (Oleszek et al., 1990b) and diosgenin glucoside and galactoside (Takechi & Tanaka 1991). Medicagenic acid glucoside with glucose at C-3 showed however, much higher activity than similar glycoside substituted with glucuronic acid. Prolongation of the sugar chain in monodesmosides could lead to a gradual decrease in activity. Comparison of hemolytic and antifungal activities of partial acid hydrolysates of dioscin and dioscinin showed that the activities were in general proportional to number of sugar residues, but compounds with branched sugar chain showed higher activities than those with straight chains. The substitution of aglycone with glucose at position C-3 was indicated to be
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important for antifungal activity. It is of interest to notice that even pattern of linkage of two sugars had influence on activity with Rha(1-2)Glc contributed more that Rha(1-4)Glc (Takechi et al., 1991). In the studies of α-hederin from Hedera rhombea it was documented that terminal rhamnose is very important for the antifungal activity of saponin. Methylation of carboxyl was more important for hemolytic than for antifungal activity (Takechi & Tanaka, 1990). A number of structurally divergent saponins from alfalfa (Medicago sativa) have been tested for their activity against Trichoderma viride (TABLE 3) (Oleszek et al., 1990b, Bialy, 1998). It was shown that bidesmosidic analogues of medicagenic acid were less active than monodesmosides with the activity gradually declining as the number of sugar residue in saponin molecule increased. The same trend was found for the 3-O-glucuronide medicagenic acid and its bidesmoside. However, all glucuronic acid substituted at C3 glycosides were much less active than their analogues with glucose linked at C3. However, no straight correlation between sugar number and activity could be found. The 16-OH derivative of medicagenic acid, the zanhic acid tridesmoside was totally inactive in the range up to 100 mg/ml in spite of the fact that bidesmosidic medicagenic acid glycosides with the same number of sugars had IA50 104 µg/ml (TABLE 3). Monodesmosidic saponin, 3-Glc-Glc-Glc zanhic acid, released after basic hydrolysis of tridesmoside showed IA50 around 65 mg/ml. Similar effect of reduction of antifungal and hemolytic activity has been observed for 17-OH derivatives of dioscinin (Takechi et al., 1991). C. Antiviral activity Most of the work that has been performed on antiviral activity of plant saponins did not exceed the experimental level. Some of the studies are listed in TABLE 4. The most frequently studied compound was glycyrrhizin (FIGURE 5), which was shown to inhibit some DNA and RNA viruses in vitro and to have therapeutic and prophylactic effects on some chronic viral hepatitis (Pompei et al., 1979). This compound was shown to inhibit the growth of several enveloped viruses including varicella-zoster virus (VZV), giving 100% inhibition of cytopathic effect (CPE) at the concentration 5.33 µg/ml, human immunodeficiency virus (HIV) (IC50 = 404 mg/ml) and VZV (IC50 = 584 µg/ml). This did not affect naked virus (poliovirus type 1). Glycyrrhizin had no direct inactivation effect on virus particles, and no interferon inducing activity in vitro or in vivo. Its biological activity is believed to be related to the action of one or more steps of the viral replication cycle. Similar results were obtained by Aquino et al. (1996) for the number of triterpene saponins including quinovic acid and oleanolic acid glycosides. The infection by enveloped virus (VSV) was generally more sensitive to these glycosides than infection by naked virus (HRV). However, much lower concentrations were required for plaque reduction (MIC50 ranged from 20 to 60 µg/ml). The most effective of quinovic acid glycosides was the compound with unsubstituted -COOH groups at C-27 and C-28 (MIC50 = 20 µg/ml, CD50 = 100 mg/ml). No correlation was found between the activity against VSV and the number of sugars in glycoside molecule. Several oleanolic acid glycosides were tested against HRV and VSV infection on HeLa and CER cells, respectively. The maximum non-toxic concentration ranged from 4 to 12 µg/ml was found for compounds having free carboxyl groups, while their esters showed reduced activity. The HRV was reduced affected only by one glycoside (De Tomassi et al., 1991).
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TABLE 3: Inhibitory activity (IA50) of alfalfa root medicagenic acid glycosides against T. viride Compound
IA50 (µg/ml)
3-Glc 3-Glc, 28-Glc 3-Glc-Glc, 28-Glc 3-Glc, 28-Ara-Rha 3-Glc-Glc-Rha 3-Glc-Glc-Glc, 28-Glc 3-Glc, 28-Ara-Rha-Xyl 3-Glc-Glc, 28-Ara-Rha-Xyl 3-Glc-Glc-Glc, 28-Ara-Rha-Xyl 3-Glc-Glc-Glc, 28-Ara-Rha-(Api)-Xyl 3-GlcA 3-GlcA, 28-Ara-Rha-Xyl
1.6 33.0 68.0 42.0 40.0 94.0 13.5 35.0 64.0 104.0 9.1 47.5
Based on Oleszek et al., 1990b, Bialy, 1998
The steroidal spirostane saponins, dioscin and gracillin, both having diosgenin (FIGURE 5) as an aglycone are cyctotoxic above 4 and 20 mg/ml, respectively and do not give interesting results below these concentration in the antiviral screening using VSV and HRV-1B. Furostanol glycosides are less cytotoxic and the compounds with 25R configuration gave 100% plaque reduction at 100 mg/ml but were less active against HRV. The opposite was found for compounds with 25S configuration, which were active against HRV, which cytopathic effect is reduced to 25% at 4 mg/ml. It was strongly stressed that 25R and 25S epimers give an inverted intensity of action against enveloped and naked viruses (Aquino et al., 1996). In the studies of Akhov et al., (1999) on the effect of steroidal furostanol saponin known under its common name as deltoside, isolated from underground parts of Allium nutans was tested against tobacco mosaic virus (TMV). The virus was treated with 0.6, 1.25 and 2.5 µg/ml solutions of saponin and after 30 min it was put on the grid and observed with electronic microscope (FIGURE 6). It was shown that saponin caused the agglutination of virons and creation of knots and fibrils on the surface of the virus. Interesting data were published by Okubo et al., (1994) on the activity of saponins having soyasapogenol as an aglycone. These saponins are quite common in legume seeds and most dominant is soyasaponin I (FIGURE 5), the triterpene saponin related in the structure to glycyrrhizin. They have partial inhibitory effect on HIV- induced cytopathology in infected MT-2 lymphocyte cultures (Nakashima et al., 1989). They also completely inhibited HIV- induced cytopathic effects and virus specific antigen expression 6 days after infection at the concentration higher than 0.25 mg/ml (Okubo et al., 1994). This saponins inhibit virus replication during an early stage of replicative cycle, i.e. adsorption or penetration of HIV, and in this respect might be a very promising specific for preventing a large number of healthy carriers from developing AIDS. It seems that soyasaponin I causes no side effects and is naturally present in legume seeds, a very important source of protein in the diet of oriental people.
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TABLE 4. Antiviral activity of saponins Saponin
Plant Source
Virus type
Chikusetsusaponin III Deltoside Extract MeOH Extract Glycyrrhizin
Panax japonicum Allium nutans Mimosa hamata Verbascum thapsiforme Glycyrrhiza glabra
HSV-1 TMV
Holoturinosides Oleanolic acid glycosides
Holothuria forskalii Calendula arvensis
Protoprimulagenin glycosides
Anagalis arvensis
Quinovic acid glycosides
Uncaria tometosa Guettarda platypoda
Rosamultin, Kajiichigoside F1 Saikosaponin a Soyasaponin (Bb) Soyasaponin I and II Soyasaponin B1 and B2 Spirostane and furostane glyc.
Bupleurum falcatum Glycine max Glycine max Glycine max Tamus communis Asparagus cochinchinensis
Reference
Fukushima et al., 1995 Akhov et al., 1999 Jain et al., 1997 HSV-1 Slagowska et al., 1987 HAV Crance et al., 1990 VZV Baba & Shigeta, 1987 HIV-1 Ito et al., 1987 HIV-1, HSV-1 Hirabayashi et al., 1991 HIV Hattori et al., 1989 HIV-1 Hasegawa et al., 1994 VSV Rodrigues et al., 1991 VSV, HRV De Tomassi et al., 1991 HRV-1B, VSV Aquino et al., 1996 HSV-1, AV-6, Amoros et al., 1987 VSV Amoros et al., 1988 HRV-1B, VSV Aquino et al., 1996
HSV HIV-1 HSV-1 HIV HRV-1B, VSV
Taurosid I
HIV-1
Tormentic acid, euscafic acid
HSV-1, poliovirus
Rucker et al., 1991 Ushio & Abe, 1992 Okubo et al., 1994 Hayashi et al., 1997 Nakashima et al., 1989 Aquino et al., 1996 Krivorutchenko et al., 1997 Simoes et al., 1990
Oleanolic acid glycosides Triterpene saponins Triterpene saponins
Chenopodium anthelminticum
Influenza A2 Influenza A2
Rao et al., 1974 Vichkanova and Goryunova, 1971
Zingibroside R1
Callistephus chinensis Glycyrrhiza glabra Panax zingiberensis
HIV-1
Hasegawa et al., 1994
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FIGURE 6. A micrograph of tobacco mosaic virus treated with 1.25 µg/ml solution of deltoside, furostanol saponin from Allium mutans.
V. BIOLOGICAL ADVANTAGE A. Additive advantage to foods Saponins can be found as ingredients of many plants used as a human food. Some of the most important have been listed in TABLE 5. The knowledge about these compounds as food components has increased substantially during last few years. It has been documented that they are generally not absorbed in the digestive tract and thus, do not create serious toxicological problems. Hemolytic and toxic effects in fish and high toxicity to invertebrate pests are well known. Oral toxicity of saponins has been estimated to be low (Price et al., 1987). Ingestion of saponin containing food by man and animals has been associated with both deleterious and beneficial effects; the former resulting in reduced weight gain in animals fed for example alfalfa, and the latter their purported hypocholesterolemic effect. It is not clear what mechanism reduces weight gain in animals, but it is generally agreed that the responsible factor is not toxicity but rather bitterness of saponins, resulting in reduced feed consumption. However, some of these effects may be attributed to the ability of saponins to affect membrane integrity. Studies of a number of saponins showed that the features which appear to be necessary to produce a permeabilizing effect are a combination of type and the number of sugar chains per molecule in addition to the nature of the aglycone to which these sugars are attached (Gee et al.,1998). Preliminary data obtained by computer modeling showed that saponin molecules can have cage-like shapes, which appear to be related to their ability to reduce
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TABLE 5. Saponin content (%) of various food plants Plant source Peanuts Millet Alfalfa sprouts Spinach root Horse chesnut Guar Oats Sesame seeds Asparagus Garlic Lentils Pea products Bean products Soybean products
Saponin content (%) 1.3 - 1.6 0.02 0.6 4.7 3-6 10 0.1 0.3 1.5 0.3 0.11-0.46 0.01-0.51 0.02-3.3 0.15-0.6
Adapted from Price et al., 1987
potential difference across the intestinal epithelium, which is thought to reflect a loss of membrane integrity affecting some or all of the mucosal cells, possibly as a result of formation of stable micelle-like structures in cell membrane. Such intestine “holes” may permit food toxins and xenobiotics to be easily absorbed. The beneficial effect of saponins reflects their abilities to bind diet cholesterol. Saponin-cholesterol sandwich-like insoluble, nondigestible macromolecules are formed in digestive tract, which in turn significantly prevent the absorption of bile salts from the perfused small intestine (Oakenfull, 1981). It has been documented that saponins reduce diet-induced hypercholesterolemia in rats and lead to the significant increases in fecal exertion of neutral sterols and bile acids (Oakenfull et al., 1983). The authors suggest that particular saponins reduce hypocholesterolemia by different mechanisms. It has been suggested that alfalfa and Quillaya saponins reduce the primary absorption of dietary cholesterol, while saponins derived from Saponaria and soybean increase fecal excretion of bile salts. The discovery that some saponins are hypocholesterolemic has provoked considerable research and clinical interest. Malinow and co-workers (1981) observed a regression of aortic and coronary atherosclerosis in macaques (Cynomolgas macaques) fed 1% isolated alfalfa root or 0.6% alfalfa top saponins without any side effects. The main problem in application of saponins as a cholesterol reducing formula is the fact that many inconsistent opinions can be found in literature on their effects as well as on the toxicity. The main reason is the fact that much research has been performed on extracts or very poorly defined mixtures due to difficulties with separation of single pure compounds. B. Physiological advantage to host The glycosylation process that takes place in plants is generally regarded as a means for increasing solubility of the compound, allowing saponin transport. From the other side, it can be regarded as deactivation of active aglycone to protect cell organelles. The activation can be performed when the producing organism needs protection. Thus, damage of the plant tissue may release appropriate enzymes that are able to hydrolyze bidesmosidic saponins to more active monodesmosidic forms. In this respect saponins © 2000 by CRC Press LLC
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appear to be an exception among plant antifungal compounds since even monodesmosidic compounds are polar, while the majority of other antifungal natural compounds tend to be strongly lipophilic and inactive in glycosidic forms. The Hedera helix which is rich with inactive bidesmosidic hederasaponin C contains also enzyme hydrolyzing ester linked sugar moiety to produce highly active monodesmosidic α-hederin (Schlosser, 1973). Avena sativa leaves contain inactive bidesmosidic furostanol saponins avenocoside A and B, which on tissue damage are hydrolyzed by ß-glucosidase removing glucose at C-26 and converting them to active monodesmosidic forms (Luening & Schloesser, 1976). However, the plant cell can be disrupted by the endogenous saponin as well, the case we face in in vitro activity tests. In the studies on membranolytic action of different saponins on mycelium of Botrytis cinerea and Rhisoctonia solani it was documented that digitonin, α-hederin and tomatine caused considerable leakage of free amino acids while aescin and thea saponin were less effective (Segal & Schloesser, 1975). Another saponin, cyclamin, also significantly damaged cell membranes but the effect was selective to some microorganisms. Disruption of cell membrane was accompanied by enzymatic conversion of saponins into their corresponding aglycones. The hydrolysis of the aglycone can, however, in some cases provide a protection for the fungi. Intramural ß-glucosidase in Drechslera avenacea can hydrolyse monodesmosidic 26-deglucoavenacosides A and B into aglycone nuatigenin, which due to the low water solubility precipitates and is not able to reach fungal plasma membrane (Luening & Schloesser, 1976). The same was true for tomatidine released from tomatine by Altenaria species pathogenic to the tomato fruit; non-pathogenic Altenaria species do not have such an enzymatic inactivation system (Schloesser, 1977). Some plant fungi do not produce extracellular enzymes that degrade saponins, but still can grow on the medium containing such a saponin. The best examples are Phyllostica concentrica and Pestalotia microspora, microspora of which can grow in ivy leaves in spite of not having such an enzyme. It was suggested that these fungi produce other substance(s) inhibitory to enzymes converting bi- to monodesmosidic forms (Schloesser, 1973). Some fungi can avoid saponin toxicity by invading plant parts low with these compounds. Artificial inoculation of Botrytis cinerea revealed that the fungus can only develop on the stems but not on the leaves of Cyclamen persicum (Schloesser, 1971). This difference can be explained by the cyclamin content of the respective organs. The ability of a phytopathogenic fungi to detoxify plant saponins may suggest that saponin detoxification determines the host range of these fungi (Bowyer et al., 1995). The cucurbitacin I, triterpene saponin from some Cucurbitaceae, was shown to play a protective function against Botrytis cinerea. Cucurbitacine I, when applied to cucumber fruits or cabbage leaves prior to inoculation, prevented fungus infection of these tissues. The protective effect was not due to the induction of lignification, but appeared to be caused by inhibition by cucurbitacin I of laccase formation by Botrytis (Bar-Nun & Mayer, 1990).
VI. APPLICATIONS Several plant sources have been commercially used (TABLE 6) but only two of them are actually permitted as food additives. These are Quillaya saponaria and Yucca schidigera extracts, containing triterpene and steroidal saponins, respectively. They are regarded as GRAS (generally recognized as safe) products. In the UK the use of Quillaya
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extracts in food was permitted as early as 1962; in beverages, the use of such extracts as emulsifiers and foaming agents was restricted to not more than 20 ppm by weight. These two extracts are also permitted in the USA by the FDA for use in food and beverages. They are used as a flavor enhancer in some categories of beverages including root beer, flavored teas and juices and additions to non-fat dairy products such as chocolate milk and vanilla pudding. As natural emulsifiers they have been used to emulsify oil-based flavors for candy, to prevent precipitation in a protein containing liquid composition, to prevent oil separation in mayonnaise, for use as a leavening agent in the bakery industry, to disperse oil in water type emulsion composition, to increase stability of cream when added to coffee and as a natural dispersing agent for waxes used in food coatings. They can also play an important function as natural preservatives against certain strains of bacteria (E. coli, Staphylococcus aureus, Salmonella, Pseudomonas aeruginosa) and fungi (Aspergillus niger, Penicilium chrysogenum). A recent patent claims that a simple process using Quillaya and Yucca saponins removes up to 83% of the cholesterol from the milk, 77% from cream, 80% from butter oil and reduces the cholesterol from liquefied eggs, or any other foodstuffs in aqueous systems. In Japan the use of Quillaya and Yucca extracts, soya bean saponins and enju saponins as emulsifiers has also been permitted, as a food additive. The important application of many steroidal saponins is their usage as starting materials for steroid hormone semi-synthesis. A majority of the steroids produced by the pharmaceutical industry and used as contraceptives are obtained by semi-synthesis from natural substances including saponins. The main saponin that has been used for a long time for this purpose was diosgenin extracted from different plant sources (see TABLE 6). A number of plant sources containing saponins are used as drugs for different ailments including: • in phlebology and proctology - Buchers broom (Ruscus aculeatus L.), Figwort (Ranunculus ficaria L. = Ficaria ranunculoides Roth.) • cough treatment - Snakeroot (Polygala senega L.), Common ivy (Hedera helix L.), Primrose (Primula veris L. = Primula officinalis (L.) Hill.) • anti-inflammatory - Licorice (Glycyrrhiza glabra L.), Common horse chestnut (Aesculus hippocastanum L.) • adaptogens - Ginseng (Panax ginseng C.A. Meyer), Siberian ginseng (Eleutherococcus enticosus Maxim) • in dermatology - Hydrocotyle (Centella asiatica L.), Urban ginseng [Mimosa tenuiflora (Willd.)], Marigold (Calendula officinalis L.) • kidney and gall stone formation - Mohave Yucca (Yucca schidigera Roezl ex Ortgies) • hypertension - green tea (Camelia sinensis L.) • premenstrual tension syndrome - soybean (Glycine max L.) • nasal and ocular delivery of insulin (Quillaya saponaria Molina) • detergents - Quillaya (Quillaya saponaria Molina), Soapworth (Saponaria officinalis L.), Soaproot (Gypsophila spp.), Mohave Yucca (Yucca schidigera Roezl ex Ortgies) Saponin extracts e.g. Yucca and Quillaya can be successfully used in animal feeding. Experiments with chicken show that addition of Yucca extract to the drinking water for broilers can reduce ammonia release from feces (Podgorski et al., 1996). In some other animals these saponins can modify nitrogen metabolism, alter rumen fermentation, show
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TABLE 6: Plant sources for industrially utilized saponins Plant source Agave sisalana Balanites aegyptica Chlorogalum pomeridianum Costus speciosus Digitalis lanata Digitalis purpurea Dioscorea composita Dioscorea terpinapensis Dioscorea spp Glycine max Quillaya saponaria Smillax spp. Solanum spp. Trigonella faenum-graecum Yucca schidigera
Common name Sisal, Henequen Soaproot, California soap plant Purple Foxglove Digitalis Yams, Barbasco
Soybean Quillaya
Fenugreek Mohave Yucca, Joshua Tree
Use Hecogenin source Diosgenin source Amolonin source Diosgegnin source Digitonin source Digitonin source Diosgenin source
Soyasaponin source Soaps, foaming agents Smilagenin/sarsapogenin source Solasodine source Diosgenin source Soaps, foaming agents
antiprotozoal activity, modify fat digestion and absorption and generally improve animal performance (Makkar & Becker, 1996). Industrial uses of saponins may include: • bleaching or de-inking agent in recycled paper industry • preventing pitch stain during the paper making process • reducing odors in municipal sewage pond systems • acceleration of microbial growth in both aerobic and anaerobic systems • coating and dispersing fat particles in waste water • suspending the silver halides in photographic films
VII. SAFETY Cytotoxicity of plant saponins precludes their practical application and some of them may show quite high cytotoxic activity (in vitro), anti-tumor (in vivo) and chemopreventive (in vitro and in vivo). These activities show concentration dependent effects and change on the structure of the aglycone and sugar substitutions. Some examples of these activities are listed in TABLE 7. Along with cytotoxic activities a number of antimutagenic activities have also been performed. Generally, saponins show no or little mutagenic activity and some antimutagenic activities. Thirteen saponins, oleanolic acid and hederagenin glycosides, isolated from Calendula officinalis, Calendula arvensis and Hedera helix were tested for toxicity and mutagenicity using a modified liquid technique of the Salmonella/microsomal assay (Elias et al., 1990). All tested saponins showed no toxicity and mutagenicity for doses of 400 µg. Screening for the antimutagenic activity was performed with two known promutagenic substances benzo[a]pyrene (MaP) and mutagenic urine concentrate from smokers (SU). Saponins showed antimutagenic activity against BaP (1µg) and SU (5µl) and the activity showed dose-response relationship. The medicagenic acid (Na+), its 3-O-glucopiranoside and soyasaponin I have been studied for their mutagenicity with the Ames test in the concentration range of 0-500 mg per plate. None of the tested compounds increased the number of his revertants in Salmonella typhimurium strains TTA97, TA98, TA100, TA102, neither in the presence or
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absence of S9 fraction from rat liver. Thus, according to Ames criterion none of the compounds was mutagenic (Czeczot et al., 1994). Some saponins e.g. glycyrrhizin and glycyrrhetinic acid, when applied at high doses for a prolonged time, show a side effect causing edema and hypertension in some patients. This side effect, called pseudoaldosteronism, is induced by the inhibitory effect of these two saponins against the reductase for mineral cortocoid in the liver resulting in retention of Na+ and water and excretion of K+.
VIII. BIOTECHNOLOGY Industrial demand for the Quillaya, Yucca and ginseng saponins requires development of the new technologies for their production. For decades, Quillaya and Yucca extracts have been produced from trees. Every year about 60,000 trees were cut causing serious ecological damage and a shortage of resources. One of the solutions is pruning the trees on the plantations. For ginseng, the predominant source is field-cultivated material. However, the field cultivation is a time-consuming and labor-intensive process subject to several additional conditions like soil, climate, pathogens and pests. The alternative to field production is plant cell culture technology. Trials with Panax notoginseng performed in China showed that bubble column reactors, air-lift bioreactors and shake flask techniques can be used for high density (23-25 g/l) cell cultivation. The biomass productivity was 1083, 146 and 916 and production of saponins was 32, 43 and 50 mg per liter per day (Zhong & Yao, 1999). Callus and cell suspension cultures of American ginseng (Panax quinquefolium) were compared for biomass growth and ginsenoside production over a 35-day culture cycle on modified MS medium. The biomass yields in suspension and callus cultures were maximal on the 25 and 30 day of growth. Both types of culture were able to produce ginsenosides in amounts and quality comparable to the cultivated plants. Appreciable amounts of ginsenosides, particularly Rg 1, were found to leach out in the culture medium of 30- to 35 day-old suspension culture (Archana et al., 1994). The production of saponins can be increased by appropriate sugar type and concentration. The culture media of Panax pseudoginseng containing 30, 60, or 100 g sucrose per liter produced on average 4.55, 37.25 and 91.83 embryoids (derived from ginseng shoots), respectively. The HPLC profile of saponin composition of the ginseng embryoids was similar to that found for the roots of naturally grown plants (Asaka et al., 1994). Cell suspension culture technique has been applied to the production of antifungal spirostanol saponins from Solanum chrysotrichum (Schldl.). Hypocotyl-derived calluses grown for 25 days in shake flasks can yield 14 mg saponins per gram, which is 50 times that of field grown plants. When grown in 10 l airlift reactor with 3g/l dry inoculum in batch culture, higher levels of biomass were achieved with cotyledon derived (14.6 g/l) than with hypocotyl derived (7.7 g/l) cells. The maximum productivity of saponins in bioreactors was 0.025 g/l/day after 9 days in culture (Villarreal et al., 1997). Oleanolic acid on an industrial scale can be obtained from sugar beet pulp after extraction of sucrose. Oleanolic acid is present in this solution in glycosidic form (glucuronide, glucoside or methylated glucoside). The ß-glucuronidase from Pseudomonas paucimobilis H-3 hydrolyzed almost all beet saponin containing glucuronic acid to produce oleanolic acid and 73% of beet saponin was hydrolyzed to oleanolic acid in 24 hours (Ishikawa, 1996). © 2000 by CRC Press LLC
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TABLE 7. Cytotoxic activity of saponins Saponin Diosgenin, dihydrodiosgenin Diosgenin glycosides
Plant Source Dracena afromontana Paris polyphylla
Diosgenin glycosides Echinocystic acid octaglyc. Ginsenoside Rb2
Balanites aegyptica Entada phaseoloides Panax ginseng
α-Hederin Holestane glycosides Oleanolic acid diglycoside Pectiniosides A-F
Hedera helix Holothuria forskalii Panax zingiberensis Asterina pectinifera
Saikosaponins Sho-saiko-to medicine Saikosaponi-acetylglycosyl Sarasinoside A1 Sarasinosides D-G
Buphlerum wenchuanese Asteropus sarasinosum Asteropus sarasinosum
Solamargine Khasianine Spirostanol glycosides Trillin Triterpene glycosides Triterpene glycosides Tubeimoside 1
Solanum spp. (Chamadeorea linearis) Dracaena afromontana Dysoxylum cumingianum Myrsine australis Bobolstemma paniculatum
Yamogenin glycosides Zingiberoside R1
Balanites aegyptiaca Panax zingiberensis
Cytotoxicity KB cells KB cells P-388 L-1210 P-388 L-5178 Y RLE, B16 HRA B 16 P-388 MT-4 L 1210 KB PLC/PRF/5 Hep-G2 P-388 P-388 A-549 HT-29 P-388 B 16-F 10 PLC/PRF/5 PLC/PRF/5 L 1210 KB cells MOLT-4 P-388 GOTO A-172 PANC-1 COLO 320 DM P-388 MT-4
Concentration 10 µg/ml 0.16-0.29 µg/ml 0.22-0.44 µg/ml 0.14-0.43 µg/ml 0.21-2.4 µg/ml 0.83 µg/ml not effective 10-100 µmol 5 mg/ml 0.38-0.46 µg/ml 46.2 µmol 8.8-11 µg/ml 10-11.5 µg/ml 20-50 µg/ml 500 µg/ml (80% Z + 20% E-ajoene ) >500 µg/ml (80% Z + 20% E-ajoene ) >500 µg/ml (80% Z + 20% E-ajoene ) 0.4 mM (49 µg/ml; allicin) 500 µg/ml (80% Z + 20% E-ajoene ) >500 µg/ml (80% Z + 20% E-ajoene ) >500 µg/ml (80% Z + 20% E-ajoene )
Effect A B A B C A C E C F G G A C A A A A D B A C A A A
Reference Naganawa et al., 1996 Yoshida et al., 1999 Naganawa et al., 1996 Yoshida et al., 1999 Chang et al. 1997 Naganawa et al., 1996 Cavallito & Bailey, 1944 Paludan-Muller et al.,1999 Sivam et al., 1997 You et al., 1998 Chung et al., 1998 Chen et al., 1999 Naganawa et al., 1996 Firouzi et al. 1998 Naganawa et al., 1996 Naganawa et al., 1996 Naganawa et al., 1996 Naganawa et al., 1996 Feldberg, et al., 1988 Yoshida et al., 1999 Naganawa et al., 1996 Sivam et al., 1997 Naganawa et al., 1996 Naganawa et al., 1996 Naganawa et al., 1996
Ajoene effects are elicited by the presence of both the disulfide bond and the sulfinyl group. Trans configuration or position of double bond reduces antimicrobial activity. Mechanism not elaborated/explored in this study. Allicin inhibits DNA synthesis, cellular replication as well as mRNA degradation and RNA synthesis. Garlic is a C-source for LAB fermentation. It increases pH and inhibits gram-ve bacteria and yeast. Garlic consumption protects against H. pylori and precancerous lesions. Decreased arylamine N-transferase (NAT) activity.
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TABLE 2: Antifungal activity of thiosulfinate compounds from garlic Fungal species
MIC (compound)
Aspergillis niger –M phase A. niger (ATCC 16404) A. flavis-M phase A. fumigatus-M phase Candida albicans C. albicans C. albicans
1:512 in broth, 1:8 serum 20 µg/ml (ajoene, 99% pure) 1:256 in broth, 1:8 in serum 1:128 in broth, 1:16 in serum 1:5,000 titer (garlic extract) 1:128 titer (garlic extract) 50-300 µg/ml-static 400 µg/ml – cidal (ajoene). 1:512 in broth, 1:64 in serum 20 µg/ml (ajoene, 99% pure) >500 µg/ml (ajoene) 1:64 in broth, 1:4 in serum 1:5,000 titer (garlic extract) 1:1,024 in broth, 1:128 in serum 1:128 in broth, 1:16 in serum 1:128 titer (garlic extract) 1:5,000 titer (garlic extract) 1:128 titer (garlic extract) 1:512 in broth, 1:64 in serum 1:512 in broth, 1:1,228 in serum 1:5,000 titer (garlic extract) 1:128 titer (garlic extract) 1:512 in broth, 1:64 in serum 1:512 titer 1:128 in broth, 1:16 in serum 1 mg/per day (allitridium) 100 µg/ml (allitridium) 1:5,000 titer (garlic extract) 1:5,000 titer (garlic extract) 400 µg/ml (ajoene) 1:5,000 titer (garlic extract) 1:5,000 titer (garlic extract) 1:1,024 in broth, 1:16 in serum 50 µM (synthetic ajoene) 25 & 50 mM for Y & M phase 1:5,000 (garlic extract) 1:5,000 (garlic extract) >500 µg/ml (ajoene) 1:64 in broth, 1:16 in serum 300 µg/ml (ajoene) 300 µg/ml (ajoene) 1:5,000 (garlic extract) 0.4% (w/w ajoene & cream) 1:1,024 (garlic extract) 1:5,000 (garlic extract)
C. albicans Y phase C. albicans (ATCC 10231) C. albicans Candida glabrata Y-phase Candida guilliermondii C. guilliermondii -Y-phase Candida krusei Y-phase Candida krusei Candida parapsilosis C. parapsilosis C. parapsilosis Y-phase Candida stellatoidea Candida tropicalis C. tropicalis Y-phase Cryptococcus albidus Cryptococcus neoformans C. neoformans Y- phase C. neoformans C. neoformans Dactulomyces crustaceus Dactulomyces floccosum Hanseniaspora valbyensis Humicola lanuginosa Microsporum spp Mucor pusillus Paracoccidioides brasiliensis Paracoccidioides brasiliensis Penicillium marneffei Phialophora pedrosoi Pichia anomala Rhizopus arrhizus Saccharomyces cerevisiae Schizosaccharomyces pombe Scopulariopsis brevicaulis, Tinea pedis Torulopsis glabrata Trichophyton spp.
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Effect
Reference
A C A A A A B
Caporaso et al.1983 Yoshida et al. 1987 Caporaso et al. 1983 Caporaso et al. 1983 Appleton & Tansey, 1975 Moore & Atkins, 1976 Barone & Tansey, 1977
A C D A A A A A A A A A A A A A A A A A D A A A E F A A D A D D A A A A
Caporaso et al. 1983 Yoshida et al. 1987 Naganawa et al. 1996 Caporaso et al. 1983 Appleton & Tansey, 1975 Caporaso et al. 1983 Caporaso et al. 1983 Moore & Atkins, 1976 Appleton & Tansey, 1975 Moore & Atkins, 1976 Caporaso et al. 1983 Caporaso et al. 1983 Appleton & Tansey, 1975 Caporaso et al. 1983 Caporaso et al. 1983 Fromtling & Bulmer, 1978 Caporaso et al. 1983 Davis et al. 1990 Shen et al. 1996 Appleton & Tansey, 1975 Appleton & Tansey, 1975 Naganawa et al. 1996 Appleton & Tansey, 1975 Appleton & Tansey, 1975 Caporaso et al. 1983 San-Blas et al. 1989 San Blas et al. 1997 Appleton & Tansey, 1975 Appleton & Tansey, 1975 Naganawa et al. 1996 Caporaso et al. 1983 Naganawa et al. 1996 Naganawa et al. 1996 Appleton & Tansey, 1975 Ledezma et al. 1996 Moore & Atkins, 1976 Appleton & Tansey, 1975
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No data from the study. Interferes with cell metabolism by: 1) inactivation of proteins by oxidation of essential thiols to a disulfide. 2) Competitive inhibition of -SH compounds (cysteine or glutathione). 3) Noncompetitive inhibition of enzyme function by oxidation of the binding to the –SH groups at the active site. Severe damage to hyphae, thickening/morphological changes of cell wall and destruction of organelles. Antimicrobial effects may result from the presence of both the disulfide bond and the sulfinyl group. Ajoene perturbs the cell membrane leading to cell lysis, which probably affects lipids in the bilayer. Ajoene induces alterations in phospholipid and fatty acid moieties. Saturated fatty acids are reduced in Y phase. Blocks thermal induced transition from M to Y phase and leads to decay of fungal structures.
A. Allicin The antimicrobial activity of garlic (Allium sativum L) was reported by Cavallito (1944) and the active component diallylthiosulfinate was named ‘allicin’. Stoll et al. (1951) confirmed that the allicin is derived from the alliin-alliinase system. Dankert et al. (1979) examined the crude juices of garlic in an agar diffusion test for their growth inhibitory effect on five gram negative and three gram positive bacterial species and two yeast species. All test organisms were inhibited by garlic juice. Addition of complexforming agents and organic matter to the crude juice reduced its activity on all test organisms. Volatile substances showed a strong inhibitory activity after exposure for 8 hours or longer at 23ºC or 37ºC. Minimal inhibition concentrations (MIC) determined in a dilution test were found to be high for gram negative bacteria and low for both yeast species. The D-values of different test organisms in undiluted garlic juice were calculated. Pseudomonas aeruginosa had a very low D-value, whilst the bacteriostatic concentration was high. This indicates a large concentration exponent of crude garlic juice for this organism. The opposite was found for Staphylococcus aureus. The antimicrobial activity of garlic extract on the oral flora of volunteers was investigated by Elnima et al. (1983). A mouthwash containing 10% garlic in quarter Ringer solution elicited a significant reduction in the number of oral bacteria. The effect of bacteriostatic concentrations of allicin (0.2 to 0.5 mM) on the growth of Salmonella typhimurium revealed a pattern of inhibition characterized by: (i) a lag of approximately 15 min between addition of allicin and onset of inhibition, (ii) a transitory inhibition phase whose duration was proportional to allicin concentration and inversely proportional to culture density, (iii) a resumed growth phase which showed a lower rate of growth than in uninhibited controls, and (iv) an entry into stationary phase at a lower culture density (FIGURE 3). Whereas DNA and protein syntheses showed a delayed and partial inhibition by allicin, inhibition of RNA synthesis was immediate and total, suggesting that this is the primary target of allicin action (Feldberg et al., 1988). Barone and Tansey (1977) demonstrated that serial dilutions of synthesized allicin showed complete fungistasis in shake cultures of C. albicans at allicin dilutions of 1 x 10-4. The aqueous extract of garlic and allicin both show a potent in vitro antibacterial activity against isolates of multiple drug-resistant Shigella dysenteriae 1, Shigella flexneri Y, Shigella sonnei and enterotoxigenic E. coli (Chowdhury et al., 1991). The minimum inhibitory concentrations of the aqueous extract and allicin against Shigella flexneri were 5 and 0.4 µl/ml, respectively. The two agents also showed potent in vivo antibacter-
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FIGURE 3. Antimicrobial effects of thiosulfinates from garlic. Salmonella typhimurium 7004 growth in L broth at 37 °C with no treatment [] or with allicin [❍] added at 91 min to a final concentration of 0.3 mM (redrawn from Feldberg et al., 1988). Bacillus cereus growth in the presence of ajoene, = control; = 10 µg/ml ajoene; = 20 µg/ml ajoene; ❍ = 30 µg/ml ajoene (redrawn from Naganawa et al., 1996). Trichophyton mentagrophytes radial growth on SG medium in the presence of allicin, ❍ = control; = 0.78 µg/ml allicin; = 1.57 µg/ml allicin; = 3.13 µg/ml allicin (redrawn from Yamada & Azuma, 1977). Paracoccidioides brasiliensis growth in the presence of increasing concentrations of ajoene, = Control; = 50 µM ajoene; = 100 µM ajoene (redrawn from San-Blas et al., 1989).
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ial activity against experimental shigellosis in a rabbit model. Oral administration of the two agents completely cured the infected rabbits within 3 days. On the contrary, 4 of the 5 rabbits in the control group died within 48 h after challenge. The experimental groups were pathogen-free on the second day of treatment. The antibacterial activity against the challenge strain was observed in the sera of the treated rabbits with 30-60 min of administration of the agents. The LD50 values of the aqueous extract and allicin in mice were 174 ml/kg and 204 µl/kg of body weight, respectively. At the therapeutic dose, the two agents did not show any adverse effects on the standard biochemical profile of blood. Using direct pre-infection incubation assays, Weber et al. (1992) reported the in vitro virucidal effects of fresh garlic extract, its polar fraction, and the following garlic associated compounds: diallyl thiosulfinate (allicin), allyl methyl thiosulfinate, methyl allyl thiosulfinate, ajoene, alliin, deoxyalliin, diallyl disulfide, and diallyl trisulfide. Activity was determined against selected viruses including, herpes simplex virus type 1, herpes simplex virus type 2, parainfluenza virus type 3, vaccinia virus, vesicular stomatitis virus, and human rhinovirus type 2. The order for virucidal activity generally was: ajoene > allicin > allyl methyl thiosulfinate > methyl allyl thiosulfinate. Ajoene was found in oil-macerates of garlic but not in fresh garlic extracts. No activity was found for the garlic polar fraction, alliin, deoxyalliin, diallyl disulfide, or diallyl trisulfide. Fresh garlic extract, in which thiosulfinates appeared to be the active components, was virucidal to each virus tested. The predominant thiosulfinate in fresh garlic extract was allicin. Lack of reduction in yields of infectious virus indicated undetectable levels of intracellular antiviral activity for either allicin or fresh garlic extract. Furthermore concentrations that were virucidal were also toxic to HeLa and Vero cells. Virucidal assay results were not influenced by cytotoxicity since the compounds were diluted below toxic levels prior to assaying for infectious virus. These results indicate that virucidal activity and cytotoxicity may have depended upon the viral envelope and cell membrane, respectively. However, the authors concluded that the activity against non-enveloped virus may have been due to inhibition of viral adsorption or penetration. Diallyl trisulfide is a chemically stable final transformation product of allicin was synthesized in 1981 in China and used for treatment of bacterial, fungal and parasitic infections in humans. Lun et al. (1994) investigated the activity of diallyl trisulfide in several important protozoan parasites in vitro. The IC50 (concentration which inhibits metabolism or growth of parasites by 50%) for Trypanosoma brucei brucei, T.b. rhodesiense, T.b. gambiense, T. evansi, T. congolense and T. equiperdum was in the range of 0.8-5.5 µg/ml. IC50 values were 59 µg/ml for Entamoeba histolytica and 14 µg/ml for Giardia lamblia. The cytotoxicity of the compound was evaluated on two fibroblast cell lines (MASEF, Mastomys natalensis embryo fibroblast and HEFL-12, human embryo fibroblast) in vitro. The maximum tolerated concentration for both cell lines was 25 µg/ml. These results indicated that diallyl trisulfide has potential to be used for treatment of several human and animal parasitic diseases. In a recent study, allicin was shown to inhibit the ability of Entamoeba histolytica trophozoites to destroy monolayers of baby hamster kidney cells (Ankri et al., 1997). Allicin has strongly inhibited cysteine proteinases, an important contributor to amoebic virulence, as well as alcohol dehydrogenase system of the parasite.
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Mechanism of action: Barone and Tansey (1977) proposed that garlic and allicin interfered with C. albicans cell metabolism by inactivation of proteins, competitive inhibition of sulfhydryl compounds, or by noncompetitive inhibition of enzyme function by oxidation. It is hypothesized that at the cidal or static levels allicin disrupts cell metabolism in Candida by inactivating proteins by the oxidation of essential thiols to a disulfide. This competitively inhibits the activity of sulfhydryl compounds by interaction with glutathione or cysteine. Noncompetitive inhibition of enzyme function is from the oxidation binding to the –SH groups at the enzyme’s allosteric sites. Candida cells in the yeast phase are more pathogenic than the mycelial form. Allicin may interfere with the electron flow through the disulfhydryl reductase system and antagonize the reductase function by oxidation of the sulfhydryl groups within the Candida cell wall. In addition, direct interference with the reductase molecule may occur. The actions may uncouple cell division from cell metabolism, resulting in an increase of mycelial forms of Candida. This effect of allicin on yeast division may decrease virulence of Candida by enhancing the conversion of the yeast form to the mycelial form (Barone & Tansey, 1977). Yamada and Azuma (1977) found allicin inhibits swelling and germination of spores at concentrations of 3.13 µg/ml or more. Normal hyphae were not observed after allicin administration in Candida albicans, Cryptococcus neoformans, Aspergillis fumigatus, Trichophyton mentagrophytes, T. ferrugineum, T. rubrum, Microsporum gypseum, and Epidermophyton floccosum. The MIC’s for Candida albicans, Cryptococcus neoformans, Trichophyton mentagrophytes, T. ferrugineum, T. rubrum, Microsporum gypseum, Epidermophyton floccosum were as low as 3.13 to6.25 µg/ml on SG agar media and 1.57-6.25 µg/ml in SG broth medium, even after 5 to 15 days after incubation (FIGURE 3). The MIC’s for Aspergillis fumigatus was 12.5 to 25 µg/ml (both broth and agar) after 5 days of incubation. It appears that allicin interferes with normal hyphae production. Allicin may affect cellular replication involving DNA and or RNA synthesis. Cellular lesions or depletion of nutrients may reset the initiator protein mass/DNA ratio required for cellular replication, in addition to being a reversible inhibitor of RNA synthesis in the cells. It is possible that allicin may affect RNA polymerase, and or possibly inhibit mRNA degradation as well as RNA synthesis (Feldberg et al., 1988). Ankri et al. (1997) determined that allicin inhibits the ability of Entamoeba histolytica trophozoites to destroy monolayers of baby hamster kidney cells. Ankri also found that cysteine proteinases (a major contributor to the amoebic virulence) as well as alcohol dehydrogenase are strongly inhibited by allicin. B. Ajoene Yoshida et al. (1987) reported the antifungal activity of six fractions derived from garlic in an in vitro system. Ajoene had the strongest activity in these fractions. The growth of both Aspergillus niger and C. albicans was inhibited by ajoene at less than 20 µg/ml. San-Blas et al. Demonstrated ajoene mediated inhibition of Paracoccidioides brasiliensis growth by 90% in the Y phase and 60% in the M form with just 50 mM of ajoene, and at 100 mM cell membrane thickened to an average of 60nm (control cells were 12 nm thick). In addition, cell membrane lysis was observed with 200 µM ajoene. During the M phase, 100 µM ajoene showed a moderate thickening of the membrane (20 nm) as well as some discontinuity and detachment of the membrane from the cell wall (FIGURE 3; FIGURE 4A & 4B).
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Naganawa et al. (1996) studied the effect of ajoene and DAD effects on fungi and bacteria. Results indicated that the anti-microbial effects may result due to the presence of disulfide bond and sulfinyl group in each compound. Fungicidal effects were found against Candida albicans, Hanseniaspora valbyensis, Pichia anomala, Schizosaccharomyces pombe, and Saccharomyces cerevisiae, and bactericidal effects were observed against Bacillus cereus, Bacillus subtilis, Staphylococcus aureus, Mycobacterium smegmatis, Mycobacterium phlei, Micrococcus luteus, Lactobacillus plantarum, Streptococcus sp., Streptomyces griseus, Escherichia coli, Klebsiella pneumoniae, Xanthomanas maltophilia, and Pseudomonas aeruginosa. The minimal microbicidal concentrations (MMC) for the bacteria were found to be: Bacillus cereus (300 µg/ml) (FIGURE 3), Bacillus subtilis (>500 µg/ml) Staphylococcus aureus (400 µg/ml), Mycobacterium smegmatis (>500 µg/ml), Mycobacterium phlei (>500 µg/ml), Micrococcus luteus (>500 µg/ml) , Lactobacillus plantarum (not determined), Streptococcus sp. (> 500 µg/ml), Streptomyces griseus (>500 µg/ml), Escherichia coli (400 µg/ml), Klebsiella pneumoniae (> 500 µg/ml), Xanthomanas maltophilia (> 500 µg/ml) Pseudomonas aeruginosa (no inhibition found up to 500 µg/ml concentration). The MMC for yeast was found to be >500 µg/ml for Candida albicans, Hanseniaspora valbyensis (400 µg/ml), Pichia anomala (>500 µg/ml), Schizosaccharomyces pombe (300 µg/ml), Saccharomyces cerevisiae (300 µg/ml). The effective mixture of ajoene consisted of a solution of 80% Z-ajoene and 20% E-ajoene. Ajoene also exhibits a broad-spectrum antimicrobial activity (Naganawa et al., 1996). Growth of gram-positive bacteria, such as Bacillus cereus, Bacillus subtilis, Mycobacterium smegmatis, and Streptomyces griseus were inhibited at 5 µg/ml of ajoene. S. aureus and Lactobacillus plantarum also were inhibited below 20 µg/ml of ajoene. For gram-negative bacteria, such as E. coli, Klebsiella pneumoniae, and Xanthomonas maltophilia, MICs were between 100 and 160 µg/ml. Ajoene also inhibited yeast growth at concentrations below 20 µg/ml. The microbicidal effect of ajoene on growing cells was observed at slightly higher concentrations than the corresponding MICs. B. cereus and Saccharomyces cerevisiae (105 cfu/ml) were killed at 30 µg/ml of ajoene in 24 h. However, the MIC for resting cells were at 10 to 100 times higher. The disulfide bond in ajoene appears to be necessary for the antimicrobial activity of ajoene, since reduction by cysteine, which reacts with disulfide bonds, abolished its antimicrobial activity. Recently, Yoshida et al. (1998) isolated a compound showing antimicrobial activity from an oil-macerated garlic extract by silica gel column chromatography and preparative TLC. On basis of the results of NMR and MS analyses, the compound was identified as Z-4,5,9-trithiadeca-1,6-diene-9-oxide (Z-10-devinylajoene; Z-10-DA). Z-10-DA exhibited a broad spectrum of antimicrobial activity against gram-positive and gram-negative bacteria as well as yeasts. The antimicrobial activity of Z-10-DA was comparable to that of Z-ajoene, but was superior to that of E-ajoene. Z-10-DA and Z-ajoene are different in respect of substitution of the allyl group by the methyl group flanking a sulfinyl group. This result suggests that substitution by the methyl group would also be effective for the inhibition of microbial growth. Further studies have shown newly identified organosulfur compound from oil-macerated garlic extract and its antimicrobial effect against B. cereus, B. subtilis, S. aureus, and yeast at concentrations less than 100 µg/ml, but not against gram negative bacteria. From the results of NMR, IR and MS analyses, the structure was determined to be E-4,5,9-trithiadeca-1,7-diene-9-oxide (iso-E-10-devinyl
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FIGURE 4A. Electron microscopy of P. brasiliensis Y Phase. Thin sections: (a) control, (b) 50 µM ajoene, (c) 100 µM ajoene (bar, 200 nm). Observe the thickening and disturbance of the cell membrane with increasing amounts of ajoene. Freeze-itching: (e) control, (f) 100 µM ajoene (bar, 600 nm). An irregular fracture plane is evident in the presence of ajoene. Abbreviations: CW, cell wall; PM, cytoplasmic membrane; PS, periplasmic space; OB, osmiophilic body; E, E face of the membrane (Reproduced with permission from the American Society for Microbiology; San-Blas et al., 1989).
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FIGURE 4B. Electron microscopy of P. brasiliensis M Phase. Thin sections: (a) control, (b) 50 µM ajoene, (c) 100 µM ajoene, (d) 200 µM ajoene. Thickening of the membrane is present at an ajoene concentration of 200 µM. Freeze-itching: (e) control, (f) 100 µM ajoene (bar, 200 nm). No important changes are observed in the membrane structure. Abbrebiations are as in Figure 4A. (Reproduced with permission from the American Society for Microbiology; San-Blas et al., 1989).
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A
D
B
E
C
F
FIGURE 5A. Effect of ajoene on Y-to-M dimorphism of P. brasiliensis. (a) - (c) Control cultures transforming at 0, 24, and 48 h, respectively. (d) - (f) Culture left to transform in the presence of ajoene, at 0, 24 and 48 h, respectively. Bar = 25 µm. (Reproduced with permission from San-Blas et al., 1993).
ajoene, iso-E-10-DA). This organosulfur compound was found to be different than E4,5,9-trithiadeca-1,6-diene-9-oxide (E-10-devinylajoene, E-10-DA). (The position of the double bond in the seventh position instead of the sixth position is the difference.) Yoshida et al. (1999), determined that compound is inferior to E-ajoene, Z-ajoene and Z-10-DA, and suggested that the position of the double bond reduced the antimicrobial activity. Mechanism of action: San-Blas and co-workers (1997) reported that ajoene could induce alterations in phospholipid and fatty acid moieties, reducing phosphatidylcholine (PC) in both Y and phases of Paracoccidioides brasiliensis. PE increased to 38% in the yeast (Y) phase and 44% in the mycelial (M) phase, suggesting and inhibition of
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A
D
B
E
C
F
FIGURE 5B. Effect of ajoene on M-to-Y dimorphism of P. brasiliensis. Descriptions as in FIGURE 5A. (Reproduced with permission from San-Blas et al., 1993).
PC synthesis. The saturated fatty acids 16:0 and 18:0 were reduced in the Y phase from 67 to 35% with increase in unsaturated components. This phenomenon was not observed in the M phase. Ajoene also seems to block the thermally induced transition from M to Y phase, and disturb the membrane, leading to deterioration in the fungal structures (FIGURE 5A & 5B). In earlier studies, San-Blas et al. (1989) proposed that ajoene could cause perturbations in the cell membrane leading to cellular lysis and subsequent deterioration of all fungal structures. In addition, ajoene was taken up by the fungus, and seemed to affect the lipids in the bilayer. In eucaryotic studies with Trypanosoma cruzi, Urbina et al. (1997)
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also indicated that ajoene altered the phospholipid composition of T. cruzi epimastigotes and amastigotes. Yoshida et al. (1987) observed hyphae damage in Aspergillis niger (ATCC 16404) and Candida albicans (ATCC 10231) as well as damage to the cellular organelles. These morphological changes to the cell and destruction to the organelles suggests that ajoene has a multifactorial mechanism rather than a single mechanism in the cell. Ajoene was found to be more effective in inhibiting fungi growth than allicin at the concentration of 20 µg/ml. Trans configuration or position of double bond reduces antimicrobial activity of garlic. Yoshida et al. (1999) found E-4.5.9-trithiadeca-1,7-diene-9-oxide to be less effective than the Z- formation against Bacillus cereus, B. subtilis, Staphylococcus aureus. C. Diallyl disulfide (DADS) and diallyl sulfide (DAS) DADS and DAS could decrease arylamine N-transferase (NAT) activity in bacteria. Chen (1999) reported a decreased NAT activity in Klebsiella pneumoniae with increased levels of DADS and DAS, decreasing Km and Vmax of NAT. Chung (1998) also reported dose-dependant effects with DAS or DADS treatment with viability studies and decreased Km and Vmax of arylamine NAT enzymes of H. pylori. Klebsiella pneumoniae growth and NAT activities were decreased with increased levels of DAS or DADS. This was demonstrated in growth studies and cytosol examinations (Chen et al., 1999). Naganawa.et al. (1996) described the effects of DAD on fungi and bacteria similar to that of ajoene (see above in ajoene section). Nok et al. (1996) found DADS inhibits procylic forms of Trypanosoma brucei brucei as well as inhibiting phospholipases from T. conglense, T. vivax, and T. brucei brucei.
VI. BIOLOGICAL ADVANTAGE A. Additive advantage in foods The U.S. Food and Drug Administration (FDA) has already approved DADS for food use and it has GRAS status (by the Flavor and Extracts Manufacturers Association) for use as a synthetic flavoring substance. The Council of Europe lists it as a substance that can be added to food without being a hazard to the public’s health (Ford, 1988). Paludan-Muller (1999) suggested that garlic has a dual role in Thai low-salt fermented fish products: 1) as a substrate for fermentation, and 2) as an inhibitor of gramnegative bacteria and yeasts. Presence and proliferation of LAB proved essential for rapid pH reduction. Garlic provided a more important role than rice starch during fermentation in ‘som-fak’, when a garlic-fermenting strain of L. plantarum was identified. B. Physiological advantage to host Garlic has attained a firm place in folk medicine for centuries. In addition to antimicrobial properties, garlic could elicit multifunctional effects to benefit human health. Garlic is capable of lowering blood cholesterol and reducing secondary vascular changes. It also raises fibrinolytic activity and inhibits thrombocyte aggregation. Therefore, garlic contains highly active therapeutic principles which appear to be particularly suitable for prophylaxis of arteriosclerosis (Ernest, 1981).
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Allicin inhibits human platelet aggregation in vitro without affecting cyclooxygenase or thromboxane synthase activity or cyclic adenosine monophosphate levels (Mayeux et al., 1988). Allicin does not alter the activity of vascular prostacyclin synthase. However, it inhibits ionophore A23187-stimulated human neutrophil lysosomal enzyme release. In vivo, allicin dilates the mesenteric circulation independent of prostaglandin release or a beta-adrenergic mechanism. Garlic has been claimed to be effective against diseases, in the pathophysiology of which oxygen free radicals (OFRs) have been implicated. Effectiveness of garlic could be due to its ability to scavenge OFRs. Prasad et al. (1995) investigated the ability of allicin contained in the commercial preparation ‘garlicin’ to scavenge hydroxyl radicals (•OH) using high pressure liquid chromatographic (HPLC) method. The •OH radical was generated by photolysis of H2O2 (1.25-10 µmoles/ml) with ultraviolet light and was trapped with salicylic acid which is hydroxylated to produce •OH adduct products 2,3and 2,5-dihydroxybenzoic acid (DHBA). H2O2 produced a concentration-dependent •OH as estimated by •OH adduct products 2,3-DHBA and 2,5-DHBA. Allicin equivalent in ‘Garlicin’ (1.8, 3.6, 7.2, 14.4, 21.6, 28.8 and 36 µg) produced concentration-dependent decreases in the formation of 2,3-DHBA and 2,5-DHBA. The inhibition of formation of 2,3-DHBA and 2,5-DHBA with 1.8 µg/ml was 32.36% and 43.2% respectively while with 36.0 µg/ml the inhibition was approximately 94.0% and 90.0% respectively. The decrease in •OH adduct products was due to scavenging of •OH and not by scavenging of formed •OH adduct products. Allicin prevented the lipid peroxidation of liver homogenate in a concentration-dependent manner. These results suggest that allicin scavenges •OH and ‘garlicin’ has antioxidant activity. Chen et al. (1999) demonstrated the decrease in arylamine N-acetyltransferase (NAT) activity in Klebsiella pneumonae as well as showing that DADS and DAS inhibited NAT activity in human colon tumor cells (adenocarcinoma). Zheng et al. (1997) recently reported the inhibitory effects of allicin on proliferation of tumor cells. The effect was associated with the cell cycle blockage of S/G2M boundary phase and induction of apoptosis. You et al. (1998), in their epidemiological studies found garlic consumption to be protective against Helicobacter pylori and precancerous lesions. Gallwitz et al. (1999) proposed that the anti-parasitic and cytostatic actions of ajoene may be partially due to the many different effect of enzymes such as human glutathione reductase(GR) in the antioxidant thiol metabolism. It was found that ajoene is a covalent inhibitor and a substrate of GR. A crystal resolution structure of GR inhibited by ajoene demonstrated a mixed disulfide in the active site. This modified enzyme increased oxidase activity as compared to the free GR. This leads to the formation of single-electron reduced products resulting in superoxide anion radicals, which could damage the cells by oxidative damage. Intraperitoneal administration of radioactive labeled DADS in mice indicated a rapid uptake of the compound by liver during the first 30 minutes and highest after 90 minutes. Liver cytosol contained more than 70% of the radioactivity after 2 hours, and 80% was found as sulfates and 8% as unchanged DADS. (Pushpendran et al., 1980).
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VII. APPLICATIONS Garlic is firmly entrenched in folk medicine. Garlic has been used, at one time or another to treat problems such as asthma, coughs, heart problems, regulation of blood pressure, as a cholesterol lowering agent, for increased circulation, impotence, diabetes, cancer, lung disorders (breathing in a combination of water, vinegar and garlic steam), epilepsy, dropsy (in a poultice), hysteria (held under the nose and sniffed), leprosy, smallpox (in a poultice), vermiferge (ingested orally), rheumatism, healing cuts (placing crushed garlic in the wound), baldness (in wine for a topical lotion), and as a digestion aid. Garlic is also widely used as a flavoring agent in cooking, and is used in the cuisine of most cultures. A. Food preservative Naganawa et al. (1996) suggested a potential role for ajoene as an antimicrobial food preservative based on studies with B. cereus. A concentration of 100 µg/ml of ajoene was required to inhibit growth compared to 1 mg/ml of sorbic acid. An alternative method to preserve raw buffalo milk was reported by Jandal (1998) using lactoperoxidase, garlic extract and ethanol. This system uses the oxidation of sulfur compounds in garlic by oxygen released from the ethanol in the presence of lactoperoxidase. The oxidation products inhibit the spoilage organisms by affecting the respiratory system. Garlic juice in a 2-10% solution was effective in eliminating coliform bacteria in the first 7 days of ‘kimchi’ (fermented cabbage) fermentation (Chung et al., 1997). Mielnik (1997) conducted a study to assess the use of fresh or dried garlic as an antioxidant in frozen, de-boned chicken meat. TBA increase was more in fresh garlic than in dried garlic, and increased in all samples during frozen storage, but increases were smaller in the garlic group. In addition to the antioxidant properties, the added garlic reduced the sensory rancidity of the meat during storage. Use of garlic in mechanically de-boned meat was suggested in products where flavor and aroma are acceptable. B. Antibacterial agent Thiosulfinates from garlic are effective antibacterial agents against a variety of pathogens including: Salmonella, Listeria, E. coli, B. cereus, S. aureus, Streptococcus, Pseudomonas aeruginosa and H. pylori cause food-borne illnesses. Garlic has also been shown to inhibit various strains of food spoilage organisms (Chung, 1998; Feldberg, 1988; Firouzi, 1998; Naganawa, 1996; Sivam, 1997; Yoshida, 1999). Perhaps garlic should be considered as both a food and a non-restricted preservative. C. Antifungal agent Moore and Atkins (1976) found that C. albicans was inhibited and killed in garlic extract diluted at 1:1024, at 37˚C. It appears that garlic extract is effective at body temperature and may have potential as a medical alternative to Nystatin. Barone and Tansey (1977) also observed fungistatic conditions at 50, 150, and 300 µg/ml and fungicidal at 400 µg/ml against C. albicans. Shen et al. (1996) showed that a Chinese preparation, allitridium (diallyl trisulfide), in conjunction with amphotericin B has a synergistic effect in vitro for fungal infections.
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Ledzema et al. (1996) demonstrated the efficacy of ajoene to treat short-term therapy of tinea pedia (Athlete’s foot). After 7 days of treatment, 27 of 34 patients were shown to have complete clinical and mycological cure in seven days. The remainder of the patients (seven) was cured after 7 additional days of treatment. All patients evaluated after 90 days after treatment yielded negative cultures for mycological growth. In the People’s Republic of China, commercial Allium sativum products are used as antifungal drugs to treat systemic fungal infections (Shen, et al. 1996). D. Antiviral agent Weber et al. (1992) reported in vitro virucidal effects of fresh garlic extract, its polar fraction, and the following garlic associated compounds: diallyl thiosulfinate (allicin), allyl methyl thiosulfinate, methyl allyl thiosulfinate, ajoene, alliin, deoxyalliin, diallyl disulfide, and diallyl trisulfide. Activity was determined against selected viruses including, herpes simplex virus type 1, herpes simplex virus type 2, parainfluenza virus type 3, vaccinia virus, vesicular stomatitis virus, and human rhinovirus type 2. The order for virucidal activity generally was: ajoene > allicin > allyl methyl thiosulfinate > methyl allyl thiosulfinate. Ajoene was found in oil-macerates of garlic but not in fresh garlic extracts. No activity was found for the garlic polar fraction, alliin, deoxyalliin, diallyl disulfide, or diallyl trisulfide. Fresh garlic extract, in which thiosulfinates appeared to be the active components, was virucidal to each virus tested. The predominant thiosulfinate in fresh garlic extract was allicin. Results of this study indicate ajoene may be evaluated as a possible virucide against herpes simplex virus type 1, herpes simplex virus type 2, parainfluenza virus type 3, vaccinia virus, vesicular stomatitis virus, and human rhinovirus type 2. E. Antiprotozoal agent Garlic and garlic derivatives have been shown to elicit anti-protozoal activity (Ankri 1997, Gallwitz, 1999; Nok, 1996; Urbina, 1997) in particular, against Entamoeba histolytica and Trypanosoma cruzi, T. brucei, T. congolense, T. vivax, and Trypanosoma cruzi epimastigotes and amastigotes. F. Limitations Storage of the garlic extract is a definite limitation. Many studies have shown that garlic extract loses its antimicrobial effects during storage. These losses vary as to the temperature as well as the length of time of storage. Many dried garlic preparations contain only alliin, and no allicin or ajoene. Alliin must be converted to allicin, which requires alliinase. Stomach acid denatures this enzyme, rendering it ineffective. Thus, slight to no conversion to allicin or ajoene takes place in the stomach. Fresh whole garlic allows the conversion to take place while chewing, and possibly holding it in the mouth for a longer period of time would allow the conversion to be more efficient (as well as noticeably more flavorful). Even enteric-coated garlic may not convert to the active forms in the small intestine. Allicin created in the small intestine will invariably react with cysteine, if protein-containing foods are consumed with garlic. S-allylmer captocysteine binds to allicin, preventing uptake into the bloodstream (Tyler, 1993). Block (1985) failed to detect ajoene in garlic powder, pills, oils, or extracts. It was concluded that this was most likely due to steam distillation disintegration of the compound.
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Commercially peeled cloves were found to have very high numbers of microbes as compared with freshly peeled cloves. These microbes include Leuconostoc mesenteroides, L. dextranicum, Enterobacter intermedium, E. sakazakii, Serratia liquefaciens, Kluyvera cryocrescens, and Cryptococcus neoformans per gram (Shim, 1999). Park et al. (1998) showed dry peeled garlic and root removal reduced microbial load more effectively than a wet peeling process. Washing also reduced microbial counts, and repeated washings with water at 5˚C further reduced the contaminant load. Garlic flavor may be a problem to some persons sensitive to strong flavors. Studies done with garlic show that a flavored solution of garlic in both mouth and overall were stronger with water, intermediate with 0.1% xanthan, and the lowest with 0.3% guar gum. It was found that it lowered the flavor release by 50% (Yven, 1998). It has not yet been shown if the antimicrobial or antioxidant properties are still active in the guar gum and garlic solution.
VIII. SAFETY AND TOLERANCE Studies done with oral doses of garlic show that the antifungal activity decreases in serum after 60 minutes after first presence of antifungal activity. Urine did not appear to inhibit the antifungal activity of garlic extract. These findings suggest that some factors in serum and urine may cause degradation of garlic’s active ingredients in those systems. It is possible that high serum protein (or possibly protein containing high amounts of sulfur or sulfur-containing amino acids) may bind allicin or it may inactivate it. The drop in antifungal activity in serum may be due to the high pH of the serum in the absence of CO2. When those plates were incubated in 5% CO2 the antifungal activity of the extract in the serum was noted to be slightly higher. Caporaso and co-workers (1983) also reported that the maximum tolerable dose in humans is 25 ml of the filtered extract (100 g garlic) homogenized in 10 ml of distilled water. Data from the National Toxicological Program indicates no reported toxicity in humans (Dausch & Nixon, 1990). After ingestion of fresh garlic in a maximally tolerable dose to five volunteer patients, it was apparent that it caused significant discomfort to the oral and gastric mucosa (Caporaso et al., 1984). This could limit the effectiveness of raw garlic extract as a prophylactic substance. Possibilities may exist for placing fresh garlic in a capsule form, however gastric mucosa may still be affected. A case of partial thickness burns from a garlic-petroleum jelly plaster was reported on a child, that was applied at the direction of a naturopath physician (Parish et al., 1987). As with any protein product, allergy and hypersensitivity reactions may occur. Contact dermatitis caused by occupational contact with raw garlic has been documented. Jappe (1999), in a review of literature and in a case report of a cook who contracted garlic induced contact dermatitis, determined the garlic related adverse effects to be irritant contact dermatitis, with a rare variant of zosteriform dermatitis, allergic contact dermatitis (which includes the hematogenic variant) as well as combination reactions. Eight patients in Hong Kong developed contact dermatitis after rubbing the cut end of fresh garlic into the skin to treat infections of the groin, neck, lower limb, hands or face. The patients were treated with a fluorinated topical steroid. All treatments were successful (Lee & Lam, 1991).
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Contact sensitivity of garlic and DADS of 155 patients in a patch-test showed 5.2% of all patients reacted to garlic. It was confirmed that diallyl disulfide was the sensitizing agent in the garlic (Lembo et al., 1991). It has been suggested by Brenner and Wolf (1994) that DADS and other compounds may possibly cause a type of relapsing chronic skin diseases known as pemphigus. A. Animal studies San-Blas et al. (1989) described a lack of toxicity of ajoene in mice and dogs— at levels up to 25 mg/kg. DADS toxicity in laboratory animals was determined by Ford et al. (1988) to be 0.26 g/kg (the acute oral LD50 in rats), and 3.6 g/kg (the acute dermal LD50 in rabbits). The undiluted solution produced skin abnormalities and irritant effects in the rabbit patch test at doses of 2.5, 3.75, or 5.0 g/kg for a span of 24 hours. The effect of an oily extract, possibly DADS from garlic was shown to suppress the ability of the Trypanosoma brucei parasites to infect the host in mice studies. When administered to experimentally infected mice at a dosage of 120 mg/kg per day, the trypanosomiasis subsided in 4 days. The extract also showed inhibition of the procyclic forms of Trypanosoma brucei and phosholipases from T. congolense and T. vivax. It was postulated that DADS interferes with the membrane synthesis of the parasite. B. Clinical trials After ingestion of fresh garlic in a maximally tolerable dose, it was apparent that it caused significant discomfort to the oral and gastric mucosa of the volunteer patients in the study (Caporaso et al., 1984). Adverse effects shown in Davis et al. (1990) was similar to those from eating fresh garlic. Fresh garlic effects include vomiting, diarrhea, anorexia, flatulence, weight loss, or garlicky body odor. There were no cases of anaphylaxis. One patient experienced abdominal discomfort and nausea, which depended on rate of drug delivery. The patient had symptoms at 30 mg/hour, but not at 15 mg/hour. Twenty five percent of the patients had abdominal discomfort, nausea and thrombophlebitis at the site of intravenous administration.
IX. BIOTECHNOLOGY A. Large-scale production Currently, many companies are marketing garlic extract in various forms. During large-scale production many of the thiosulfinates seem to lose their antimicrobial activity depending on the processing conditions (Block, 1985; Barone & Tansey, 1977; Caporaso et al., 1984; Tyler, 1993). Synthetic allicin has been made by a method involving the oxidation of diallyl disulfide by an equimolar amount of organic per-acid. The steps for synthetic preparation of the extract may be found under the Section: Molecular properties, of this chapter. Stoll and Seebeck (1948) found that attaching an allyl group and an oxygen atom to the sulfur atom in the amino acid cysteine forms alliin. B. Quality control Processing and storage conditions of commercial preparations of garlic extract may compromise the antimicrobial activity of garlic products. A commercial preparation
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of garlic extract was assayed and no antifungal activity was detected for either yeast or mycelial fungi (Caporaso et al.,1983). Ajoene or allicin could not be detected in dehydrated garlic powder, pills, oils, extracts or other proprietary garlic preparations (Block, 1985; Barone & Tansey, 1977; Caporaso et al., 1983). Krest and Keusgen (1999) showed two molecular forms of alliinase (53 and 54 kDa) from garlic powder, in contrast to two identical subunits in fresh garlic. This indicates that the drying process affects the alliinase in garlic powder, however, the preparation was capable of converting alliin to allicin. Commercially peeled cloves in Korea were found to have much higher numbers of microbes than freshly peeled cloves (Shim, 1999). Raw garlic can also be contaminated by Clostridium botulinum (Roever, 1998) as can garlic flavored oils (LaGrange, 1998). Large-scale producers of fresh garlic should consider risks of microbial contamination. Presently the US Food and Drug Administration does not control the quality of herbal preparations or supplements. Any quality control done in the U.S. is self-regulated.
X. SUMMARY It has been demonstrated that garlic and its derivatives may be multifunctional as well as flavorful food additives. Garlic has been used in the past and is presently being used as a medicine, curative, preservative and a flavoring agent. The recent reports of antibiotic-resistant organisms and the threat of new emerging pathogens is a global public health problem. Microbes adapt to new environment by mutation, allowing them to survive adverse conditions by natural selection. Therefore, it is suggested that alternative or synergistic therapies that offer possible solutions or prevention should be investigated. The antimicrobial properties of garlic and its derivatives have been documented for many years. It has been shown that garlic and its derivatives exhibit both cidal and statis effects. Many studies have indicated that garlic derivatives exhibit antimicrobial properties and fresh garlic appears to provide the most optimum and efficient cidal and inhibitory effects. Although garlic and its derivatives appear to be safe for consumption, assessment and protein determination for the allergen responsible for hypersensitivity reactions needs in-depth evaluation. Certain reports have indicated allergic reactions associated with garlic consumption. These preliminary indications are worthy of further research into the specific mechanisms and the effects of garlic derivatives on susceptible microorganisms. It is apparent that the conflicts reported in the studies (MIC values etc.) are due to different strains of organisms used. Determination of the most effective sulfinate concentration range to use for a specific organism or infection is another consideration. If garlic sulfinates are to be used as preservatives or as antimicrobial agents, the purification techniques and quality control methods should be standardized. Acknowledgments. We thank Dr. Gioconda San-Blas, Centro de Microbiologia y Biologia Cellular, Venezuela for providing electron micrographs for this chapter.
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Stoll, A., and Seebeck, E. 1951. Chemical investigations on alliin, the specific principles of garlic. Advan. Enzymol. 11:377. Tynecka, A., and Gos, Z. 1973. The inhibitory action of garlic (Allium sativum L.) on growth and respiration of some microrganisms. Acta Microbiol. Polon Scr. B. 5:51-62. Tyler, V.E. 1993. Garlic and Other Alliums. The Honest Herbal. Pharmaceutical Products Press. N.Y. 139143. Tyler, VE.1994. Cardiovascular System Problems-Garlic. Herbs of Choice. Pharmaceutical Products Press.New York.104-108. Walker, J.C., Lindegren, C.C., and Bachman, F.M. 1925. Further studies on the toxicity of juice extracted from succulent onion scales. J. Agri. Res. 30:175. Walton, L., Herbold, M., and Lindegren, C.C. 1936. Bactericidal effects of vapors from crushed garlic. Food Res. 1:163. Weber, N.D., Anderson, D.O., North, J.A., Murray, B.K., Lawson, L.D., and Hughes, B.G. 1992. In vitro virucidal effects of Allium sativum (garlic) extract and compounds. Planta Med. 58:417-423. Wong, R.M., Kondo, Y., Bamba, H., Matsuzaki, S., and Sekine, S. 1996. Anti-Helicobacter pylori activity in the garlic extract. Nippon Shokakibyo Gakkai Zasshi 93:688. Yamada, Y., and Azuma, K. 1977. Evaluation of the in vitro antifungal activity of allicin. Antimicrob. Agents Chemother. 11:743-749. Yoo, K.S., and Pike, L.1998. Determination of flavor precursor compound S-alk(en)yl-L-cysteine sulfoxides by an HPLC method and their distribution in Allium species. Scientia Horticulturae.75:1-10. Yoshida, S., Kasuga, S., Hayashi, N., Ushiroguchi, T., Matsura, H., and Nakagawa, S. 1987. Antifungal activity of ajoene derived from garlic. Applied and Environmental Microbiology. 53:615-617. Yoshida, H., Katsuzaki, H., Ohta, R., Ishikawa, K., Fukuda, H., Fujino, T., and Suzuki, A. 1999. An organosulfur compound isolated from oil-macerated garlic extract, and its antimicrobial effect. Biosci. Biotechnol. Biochem. 63:588-590. You, W.C., Zhang, L., Gail, M.H., Ma, J.L., Chang, Y.S., Blot, W.J., Li, J.Y., Zhao, C.L., Liu, W.D., Li, H.Q., Hu, Y.R., Bravo, J.C., Correa, P., Xu, G.W., Fraumeni, J.F. Jr. 1998. Helicobacter pylori infection, garlic intake and precancerous lesions in a Chinese population at low risk of gastric cancer. Int J Epidemiol. 27:941-944. Yven, C., Guichard, E., Giboreau, A., and Roberts, D.D. 1998. Assessment of interactions between hydrocolloids and flavor compounds by sensory, headspace, and binding methodologies. J. Agri. Food Chem. 46:1510-1514.
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L.R. Juneja T. Okubo P. Hung
Catechins
14
I. INTRODUCTION Tea has served as a popular beverage worldwide for centuries. Historians trace the first use of tea to China, in the twenty-eighth century BC. However, written documentation does not appear until the third century BC. Green tea has been considered a crude medicine in China for 4000 years. Today, tea is the second most consumed beverage in the world following water. Green tea is one of the most popular beverages in Japan and China, and its consumption accounts for about a half of all tea consumed worldwide. The tea plant is cultivated in more than 20 countries of Asia, Africa, and South America; India and China are the biggest growers, producing 672 and 600 million pounds a year, respectively (FAO, 1993). The degree of fermentation greatly affects the quality and type of tea. According to the degree of fermentation, tea is classified into three kinds: green tea (unfermented), oolong tea (semi-fermented), and black tea (fermented). Research shows that the processing of black tea destroys certain beneficial health constituents such as catechins (polyphenolic compounds) that exist in green tea due to oxidation. Green tea has been attracting many researchers from various fields exploring treatment for ailments ranging from acne to heart disease. Green tea is a powerful physiological antioxidant and a strong candidate for therapeutic and prophylactic applications. Green tea catechins (GTC) inhibit bacterial growth (Okubo et al., 1997; Fukai et al., 1991) and suppress tumors (Ji et al., 1997). Certain studies also indicated the ability of GTC to prevent oxidation of low-density lipoprotein (LDL), precursors to heart disease (Luo et al., 1997). GTC inhibits a wide range of microorganisms including cariogenic bacteria (Sakanaka, 1997), and enteric pathogens (Okubo & Juneja, 1997; Ishihara & Akachi, 1997). The volatile constituents of green tea also demonstrate antimicrobial activity against several bacteria, fungi, viruses and parasites. Several studies have shown that GTC strongly inhibits the growth of Vibrio cholerae 01, Staphylococcus aureus, Vibrio parahaemoliticus, V. minicus, Staphylococcus epidermidis, Campylobacter jejuni, Plesiomonas shigellloides (Toda et al., 1989); Streptococcus mutans (Sakanaka et al.,
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TABLE 1. Green tea catechin composition of Sunphenon® Catechin compound (+)-Catechin (C) (+)-Gallocatechin (GC) (-)-Epicatechin (EC) (-)-Epicatechin gallate (ECg) (-)-Epigallocatechin (EGC) (-)-Epigallocatechin gallate (EGCg) Total catechin content
Composition (%, w/w) 2.7 10.7 5.9 5.2 16.5 31.9 74.8
1989) or viruses such as Influenza A, Influenza B (Nakayama et al., 1993) and more than 99% growth of viruses such as Polio type 3, Echo type 9, Coxasackie B6, Reovirus type 1, Vaccinia, Herpes simplex, (John et al., 1979). The antimicrobial effect of the Sunphenon , a commercial product of GTC containing 74.8% polyphenol prepared from green tea (Camellia sinensis) by Taiyo Kagaku Co. Ltd. (Yokkaichi, Japan), was used in the most of studies reported in this Chapter. The catechin composition of Sunphenon® is shown in TABLE 1. ®
II. OCCURRENCE Tea leaves essentially contain catechins, theanine (γ-ethylamino-L-glutamic acid), and caffeine. Most of the interest has been focused on catechins based on the isoflavan structure, and these compounds comprise about 30% of the dry weight of tea flush (the growing point of the plant, consisting of the buds and immature leaves that are picked for processing). These compounds are infused with hot water or extracted with ethyl acetate from the aqueous solution. The slight astringent and bitter taste of green tea infusion is attributed to catechins. About 5% of the dry weight of black tea (10% in case of green tea) and its aqueous extracts is made up of catechins, which are simple, well-characterized isoflavonoids. GTC mainly consists of six compounds: (+)-Catechin (C); (+)-Gallocatechin (GC); (-)Epicatechin (EC); (-)-Epicatechin gallate (ECg); (-)-Epigallocatechin (EGC); and (-)Epigallocatechin gallate (EGCg). These catechins are synthesized in tea leaves through malonic acid- and shikimic acid-metabolic pathways. The content of catechin varies depending on the species of tea plant and the season for harvesting, in which, EGCg is not found in other plants and is the major catechin in green tea (Nakabayashi, 1991; Bradfield & Penney, 1948).
III. MOLECULAR PROPERTIES A. Structure Tea catechins are a class of flavonols which are C-15 compounds, and their derivatives are composed of two phenolic nuclei (A ring and B ring) connected by three carbon units (C-2, C-3 and C-4). The flavonol structure of catechin (3, 3’, 4’, 5, 7-pentahydroxylflavan) contains two asymmetric carbon atoms at C-2 and C-3. Catechins and their derivatives also have nucleophilic centers at C-6 and C-8, which are reactive with electrophilic specimens. Chemically they are highly reactive, with properties of metal chelation, oxidative radical scavenging, nitrosation inhibition, etc.
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FIGURE 1. Chemical structure of green tea catechins (GTC).
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Green tea leaves Hot water
Ethylacetate Chromatography on high-porous polystyrene gel column. Stepwise elution with methanol/H2O
Fraction 1
Fraction 2 HPLC
HPLC
GC
EGC
Fraction 3
C
EC
HPLC
EGCg
ECg
FIGURE 2. Isolation and purification of green tea catechins (GTC).
Structure, molecular formula, molecular weight (mol.wt), melting point (m.p), optical rotation [(α)D] of each component of GTC are shown in FIGURE 1 (Hergert & Kurth, 1953; Bradfield & Penney, 1948; Birch et al., 1957). B. Isolation and purification The leaves of green tea were steeped into hot water (95 ˚C) for 30 min with gentle stirring. The ratio of tea and water is set at 1:10 (w/w). The mixture was then filtered and the tea infusion is concentrated to about quarter by volume with vacuum dryer. The catechins are extracted by adding ethylacetate three times by volume to the water extract. The ethylacetate layer is then dried with cyclone-vacuum dryer to obtain the catechins. A schematic pathway of isolation and purification of GTC is shown in FIGURE 2. GTC is separated into three fractions using chromatography with a high porosity polystyrene gel column (Diaion HP-20, particle size 75–150 µm, Mitsubishi Kasei Co., Japan). A sample of 100 mg catechins dissolved in 20 ml water is applied and eluted stepwise with 100 ml of methanol/H2O = 1/5 (fractions 1 and 2) and with methanol/H2O = 2/5 (fraction 3). Elution is performed at a flow rate of 5 ml/min. Each fraction obtained above is purified using recycling liquid chromatography equipped with GS-310 (particle size 9 µm, LC-908). The mobile phase consists of acetonitrile/H2O (3/7, v/v). Elution is performed at a flow rate of 10 ml/min with monitoring at 280 nm. These components are then analyzed using HPLC Model 600E equipped with auto-sampler model 717 and programmable multi-wavelength detector model 490E (Millipore Co., USA). A sample volume of 5 µl of is injected to a Develosil ODS-P-5 column (Nomura Chemical Co., Japan); eluted with a mixture of acetic acid:acetonitrile:N, N-dimethylformamide:H2O=3:1:15:81 (v/v/v/v) at a flow rate of 0.5 ml/min. Catechins are detected at the absorbance of 280 nm.
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Treated Untreated Treated
Dental caries in humans
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Untreated
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FIGURE 3. Anticaries activity of Sunphenon® - a commercial GTC formulation. Dental caries in rats: Animals were fed with chocolate and caramel diets containing 56% sucrose with or without 0.05% Sunphenon® for 40 days. The caries scores were then counted. (Source: Sakanaka et al., 1992). Dental caries (plaque formation) in humans: Twenty-six volunteers rinsed their mouths 3 times a day with 0.05% Sunphenon® solution for 3 days. Control group rinsed with water only. The subjects did not brush the teeth during the test period.
IV. ANTIMICROBIAL ACTIVITY A. Effects on dental caries Several epidemiological studies have suggested efficacy of green tea infusion for prevention of dental caries (Onishi et al., 1978; 1981a; & 1981b). Dental caries and periodontal diseases are the main infectious diseases in the oral cavity. Streptococcus mutans and S. sobrinus play an important role in the cause of dental caries. These bacteria synthesize water-soluble and insoluble glucans by glucosyltransferase (GTase) from sucrose in foods and drinks. Water-insoluble and highly branched glucan is responsible for the bacterial cell adherence to tooth surface (Hamada & Llade, 1980). Thus, the three major factors that play a critical role in the development of dental caries are host (tooth), bacteria, and substrate (sucrose) for the bacterial metabolism. S. mutans and other microorganisms grow in the synthesized polysaccharides (glucan) and form dental plaque. These bacteria metabolize various saccharides and produce organic acids, especially lactic acid which is retained in dental plaque and the tooth is decayed gradually. Usually one cannot recognize a dental caries before it gets worse to a © 2000 by CRC Press LLC
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considerable extent. The tooth surface once plaqued is never back to the original state. Therefore, prevention of dental caries is much more important than cure of the plagued teeth. The most traditional method of decreasing cariogenic bacteria and dental plaque is use of dental brush or chemicals such as antibiotics, antibacterial substances, as well as enzyme inhibitors and their combination (Ikeda et al., 1978; Ohshima et al., 1983; Backer et al., 1983). Various plant extracts have been investigated aiming prevention of dental caries by many laboratories (Saeki et al., 1983; Okami et al., 1981). Among such phytochemicals, GTC was considered highly effective for prevention of dental caries. Several studies have confirmed that purified catechin fraction from green tea, and ECG and EGCg in particular, inhibit the growth of many bacterial species and elicit anticariogenic properties (Ahn et al., 1991; Kawamura & Takeo, 1989; Otake et al., 1991). Specifically, Sunphenon® prevented the attachment of a cariogenic S. mutans strain to hydroxyapatite and inhibited the bacterial GTase activity (Sakanaka et al., 1990; Otake et al., 1991). Our studies showed that Sunphenon® was not only effective in the inhibition the growth of S. mutans, but also against gingivitis, glucan synthesis and of cellular adherence of cariogenic streptococci. The inhibition of the growth of S. mutans and S. sobrinus was paralleled with concentration of the catechins (Sakanaka, 1997). The GC and EGC at concentration of 250 µg/ml markedly inhibited the growth of strains such as MT-8148, IFO-13955, MT-4502, MT-4532, MT-4245, MT-4251, 6715-DP, and Mfe-28 (Sakanaka, 1997). The minimum inhibitory concentration (MIC) against cariogenic bacteria of EGCg, a major component of tea catechins, was 250-1,000 µg/ml in the brain heart infusion (BHI) medium, and their growth inhibitory effects were enhanced by two-fold or more when tested in meat extract medium (Sakanaka, 1997). On the other hand, ECg and EGCg almost completely inhibited glucan synthesis at concentrations of 25-30 µg/ml, and the adherence of bacteria cells at concentration of 50 µg/ml (Sakanaka et al., 1990; 1992). In vivo experiments in a rat model were performed to evaluate the inhibitory effect of GTC on dental caries. Rats were fed with chocolate and caramel diets containing 56% sucrose with or without 0.05% Sunphenon® for 40 days. The caries scores were then measured. The results indicated that Sunphenon® administration has significantly reduced the caries score by approximately 25% (FIGURE 3 -TOP). Human clinical studies were also conducted on the preventive effect of GTC against dental plaque. The results showed that GTC significantly decreased the dental plaque formation in the volunteers who rinsed their mouth three times a day for 3 days with a solutions containing 0.05% GTC (FIGURE 3 - BOTTOM). The total number of bacteria and streptococci on the dental plaque also decreased in all the test groups. In addition, the concentration of lactic acid in saliva decreased after rinsing with the GTC solutions (Sakanaka et al., 1997; Oiwa et al., 1993). These results suggest that GTC is a potent inhibitor of dental plaque formation in the human oral cavity. Furthermore, epidemiological studies carried out in the primary schools of two typical Japanese farm villages for 5 years which required drinking a cup of tea (Bancha) after lunch, resulted in a significant decrease in the average number of caries lesions in both village groups (Onishi, 1985).
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P. gingivalis/Epithelial cells
350
C 300 250 200 150 100 50 0 0
0.5
1
1.5
2
2.5
Sunphenon conc. (mg/ml) FIGURE 4. Inhibition adherence of Porphyromonas gingivalis adherence to oral epithelial cells Epithelial cells from oral cavity were pre-treated with Sunphenon® solution. Bacterial suspension of P. gingivalis was added to epithelial cells and incubated for 60 min. The epithelial cells and adherent bacteria were observed under an optical microscope (Source: Sakanaka et al., 1996). Dose-response curve of adhesion-inhibition: Epithelial cells and P. gingivalis were incubated with Sunphenon® at various concentrations from 0.1 - 2.5 mg/ml at 37 oC for 60 min. Epithelial cells and bacteria were washed 5 times by centrifugation (1000 rpm, 3 min) with 0.1M PBS (pH 6.0). Cells were smeared on a glass slide, dried, and stained with a safranin solution. Adherent bacteria to 20 epithelial cells were counted by light microscope and the mean values were depicted.
B. Effects on periodontal disease Periodontal diseases (periodontitis) occur during middle or old age and are considered one of the major geriatric disorders. The disease is characterized by inflammatory lesions in periodontal tissues and gingivitis. Porphyromonas gingivalis, the subgingival plaque bacteria, is one of the etiological agents of periodontitis. The adherence of P. gingivalis to oral epithelial cells is the initial step in the pathogenesis of periodontitis. In vitro experiments showed that Sunphenon® at 0.1 mg/ml and above strongly inhibit the adherence of P. gingivalis to epithelial cells (FIGURE 4). Furthermore, it was also observed that GTC, especially EGCg, GCg, and ECg, strongly inhibits the adherence of P. gingivalis (Katoh, 1995; and Sakanaka et al., 1996).
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TABLE 2. Effects of GTC on growth and inhibition of enteric bacteria Strain
Bifidobacterium adolescentis E-194a B. adolescentis E-319a B. bifidum E-319a B. bifidum S-28a B. breve S-1 B. breve S-46 B. infantis S-12 B. infantis 1-10-5 B. longum E-194b B. longum Kd-5-6 Lactobacillus acidophilus ATCC-4356 L. casei ATCC-7469 L. salivarius ATCC-11741 Bacteroides distasonis B-26 B. distasonis S-601 B. fragilis M-601 B. fragilis VI-23 B. thetaiotaomicron AS-126 B. vulgatus B-24 B. vulgatus F-62 Clostridium bifermentans B-1 C. bifermentans B-4 C. butyricum ATCC-14823 C. butyricum S-601 C. coccoides B-2 C. difficile ATCC-9689 C. innocuum M-601 C. paraputrificum B-3-4 C. paraputrificum B-78 C. paraputrificum VPI-6372 C. perfringens ATCC-13124 C. perfringens B-3-7 C. perfringens B-3-8 C. perfringens B-165-16 C. perfringens C-01 C. ramosum ATCC-25582 C. ramosum C-00 Eubacterium aerofaciens S-601 E. aerofaciens S-605 E. lentum M-601 E. limosum E-1 Escherichia coli E-605 E. coli M-602 E. coli O-601 E. coli V-603
Growth
Inhibition
PYF medium
Gyorgy medium
+ + + -
+ + + + + + + + + + + -
+ + + + + + + + + + + + + + -
Test strains were obtained from the RIKEN, cultured in peptone yeast fields (PYF) medium without C-source supplementation. Gyorgy medium was supplemented with 0.5% glucose and 1% methanol extract of green tea.. The inhibitory effect of GTC was assayed by paper-disc method (8mm diameter, Toyo Roshi, Japan) containing 10 mg of GTC per disc on Brucella agar. Tests were done three times and a mean of inhibition zone of 12 mm or larger was estimated as ‘+’.
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Count (log10 bacteria/wet feces)
12
A B 9
C
6
D E
3 0
1
2
3
Administration time
4
5
6
7
Normal
Feeding time (week) FIGURE 5. Effect of Sunphenon® on human enteric microflora. Human volunteers were administrated with 1.2g Sunphenon®/day/person for 4 weeks. Bacterial enumeration was performed from fecal samples (A - Total count; B - Bifidobacterium spp.; C - Clostridium spp., D - Clostridium perfringens; E - Lactobacillus spp.
Collagenase, which is produced by P. gingivalis, breaks down collagen in the gums, weakens the periodontal pocket and eventually recedes the gums leading to gingival and periodontal diseases. The test results showed that the activity of collagenase was significantly inhibited by 50 µg/ml Sunphenon®, and the enzyme activity was almost inhibited to zero at 100 µg/ml Sunphenon®. These results suggested that Sunphenon® significantly decreased the periodontal disease by inhibiting the growth, adherence of P. gingivalis as well as suppressing the activity of collagenase. C. Effects on human enteric microflora In the human large intestine, the undigested and unabsorbed substances are subjected to react with various enteric bacteria. These bacteria and their metabolites are closely associated with nutrition, health, aging and pathogenesis of gastrointestinal diseases. For instance, lactic acid bacteria (LAB) such as Bifidobacterium and Lactobacillus spp. are known to be useful to human and animal health as probiotics. These organisms stimulate digestion and absorption of nutrients and inhibit the growth of unfavorable microbes (Hentges, 1983; Mitsuoka, 1984). On the other hand, certain clostridia such as Clostridium perfringens, C. difficile, etc. are closely associated with intestinal malfunction, that could lead to accelerated aging or causing tumors (Bokkenheuser, 1983; Godman, 1983; Gary & Sherwood, 1984). The microflora in the large intestine are always affected by external environmental factors, in which diets are the most important. For measurement of the MIC, 0.1ml of the GTC at various concentrations was added to 9.9 ml of medium containing 1.5% agar at around 60oC in a petri dish. The mixture was agitated thoroughly and solidified at 37oC. One platinum loop of the microorganism suspension, obtained from a pre-culture at 37oC overnight, was inoculated on the agar medium, and incubated at 37oC, 48 h for bacteria or at 25oC, 96 h for fungi and yeast. Brain heart infusion (BHI) was used for bacteria, and malt extract broth was used for fungi and yeast. © 2000 by CRC Press LLC
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TABLE 3. Antimicrobial spectrum of GTC against various bacteria (MIC in µg/ml) Bacterial strain
MIC
Bacterial strain
Food-borne bacilli Bacillus subtilis IFO-3007 B. cereus ATCC-14579 B. brevis IFO-3331 B. circulans IFO-13626 B. macerans JCM-2500 B. polymyxa JCM-2507
2,000 600 700 600 800 900
Escherichia coli strains E. coli O157:H7 SAKAI212 E. coli O157:H7 ATCC43895 E. coli O139-CH15 E. coli O139-CH20 E. coli K-88 E. coli IFO-3545
Thermophilic spore formers B. stearothermophilus IAM-1035 B. stearothermophilus IFO-12550 B. stearothermophilus ATCC-12980 B. coagulans JCM-2257 Clostridium thermoaceticum No-5801 C. thermoaceticum No-5802 C. thermoaceticum No-5809 C. thermosaccharolyticum No-5604
100 150 150 200 400 400 400 100
Gram +ve / -ve strains Proteus vulgaris IFO-3581 Pseudomonas aeruginosa IFO-3080 P. fluorescens IFO-13922 Serratia marcescens IFO-3046 Staphylococcus aureus IFO 12732 Lactobacillus acidophilus IAM-1043 Streptococcus lactis IFO-12546 Helicobacter pylori ATCC-43504 Propionibacterium acnes ATCC-6919 P. acnes ATCC-11828
MIC 250 250 750 500 750 750
2,000 250 300 4,000 500 1,000 2,000 500 500 600
For MIC determination, 0.1 ml of the GTC at various concentrations was added to 9.9 ml of medium containing 1.5% agar. One platinum loop of overnight-grown bacterial suspension was inoculated on the BHI agar, and incubated at 37 ˚C for 48 h. For thermophilic sporeformers, BHI and the modified thioglycollate medium were used. Culture conditions: were aerobic for Bacillus stearothermophilus (50 ˚C, 48 h), Bacillus coagulans (37 ˚C, 48 h), and anaerobic for Clostridium bacteria. (55 ˚C, 72 h).
Growth response and inhibition of bacteria isolated from human intestines were examined. The results showed that GTC promoted the growth of useful probiotic flora while it inhibited the growth of harmful bacteria such as C. bifermentan, C. difficile, C. innocuum, C. paraputrificum, C. perfringens, and C. ramosum. Ahn et al. (1991) showed that ECg and EGCg (5 mg/disk) significantly inhibited the growth of C. difficile and C. perfringens (TABLE 2). In vivo studies on human volunteers also revealed that intake of GTC 1.2 g/day/person for 4 weeks significantly inhibited the growth of harmful bacteria but did not affect the growth of useful probiotic bacteria (FIGURE 5). Other tests were also carried out to determine the MIC of GTC against various bacteria strain isolated from foods, human sources, animals, and fish. Thermophilic spore forming bacteria were also tested for GTC susceptibility (TABLE 3 & 4). The effect of GTC on the heating time required for decreasing 10% CFU of spores (D-value) of Bacillus stearothermophilus was tested. In the presence of 500 ppm of GTC, the D-value significantly decreased at all tested temperatures as compared to control sample. The inhibition rate became greater following the increase of treated temperature. The antifungal activity of GTC was also tested on the fungi and yeast such as Saccharomyces cerevisiae IFO-0203, Candida albicans IFO-1061, Rhodotorula rubra IFO-0001, Hansenula anomala IFO-0136, Kluyveromyces fragilis IFO-1963, K. lactis IFO-1090, Metschnikowia pulcherrima IFO-1678, Aspergillus niger ATCC-3275, Mucor mucedo IFO-7684, Rhizopus chinensis IFO-4745, Penicillium chrysogenum IFO-5809, P. citrinum IFO-7784, Trycophyton rubrum IFO-5807, T. mentagrophytes IFO-5466, T. mentagrophytes IFO-5809, and T. tonsurans IFO-5946. However, no marked inhibitory effect was observed, even at 4 mg/ml concentration of GTC in the media. © 2000 by CRC Press LLC
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TABLE 4: MIC (µg/ml) values for GTC against animal- and fish-borne pathogens Animal-borne pathogens Cattle Salmonella dublin L-729 Pseudomonas aeruginosa KK-1001 S. aureus KK-103 S. aureus spp. S. aureus KK-101 S. epidermidis KK-108 S. epidermidis spp. Escherichia coli K-99
MIC 4,000 500 500 1,000 1,000 500 500 >4,000
Pig Salmonella enteritidis ZK-2a E. coli K-88(Abbotstown) E. coli K-88(G-1253) E. coli K-88(MN-1) Staphylococcus pyogenes spp.
4,000 4,000 4,000 4,000 1,000
Chicken Salmonella enteritidis L-58 S. typhimurium L-413 S. infantis L-164 4,000 S. thompson L-131 S. sofia L-59 S. mbandaka L-743 S. mbandaka spp. S. huderberg spp.
4,000 4,000 4,000 4,000 2,000 4,000 4,000 4,000
Fish-borne pathogens
MIC
Ayu Vibrio anguillarum IFO-13266 V. anguillarum UP-1 V. anguillarum PT-213 V. anguillarum PT-493 Vibrio spp.
200 200 150 150 200
Crawfish Vibrio sp. PJ V. alguillarum V. fluvialis V. damsela ATCC-33539
50 400 200 200
Yellowtail Streptococcus spp. S. KS-8903 S. KS-8930 S. KS-8982 S. b-hemlosys Pasteurella piscicida spp. P. piscicida OT-8447 P. piscicida 5866
1,000 700 800 900 900 100 200 150
Eel Edwardjella tarda SH-89133 E. tarda E-2812 E. tarda SY-84006 Vibrio vulnificus ATCC-33147 V. parahaemolyticus ATCC-17802
400 300 400 200 200
Salmon Vibrio vulnificus Vibrio spp.
200 100
Other fish Aeromonas salmonisida A. hydrophila Vibrio alguillarum ATCC-19264 V. harveyi
800 200 400 100
For MIC determination, 0.1 ml of the GTC at various concentrations was added to 9.9 ml of medium containing 1.5% agar. One platinum loop of overnight-grown bacterial suspension was inoculated on the BHI agar, and incubated at 37 ˚C for 48 h.
D. Effects on Escherichia coli O157:H7 Escherichia coli O157:H7 is one of the enterohemorrhagenic pathogens. In 1993, the outbreak of hemorrhagic colitis caused by E. coli O157:H7 in uncooked hamburger meats was reported in Mermelstein (United States). The seriousness of this strain generated interest during the sensational outbreak in Japan in 1996. More than 3,000 people infected with E. coli O157:H7 seriously suffered from diarrhea with a high rate of mortality. E.coli O157:H7 produces a cytotoxin known as verotoxin or shiga-like toxin, which shows strong toxicity on vero cells. This cytotoxin causes hemorrhagic colitis and
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Natural Food Antimicrobial Systems
hemolytic uremic syndrome in humans (Karmali et al. 1985). Various laboratories have tested the efficacy of various antimicrobial systems to control E.coli O157:H7. Such systems included a wide variety of antibiotics (Hathcox et al., 1996; Podolak et al., 1996), antioxidants (Ogunrinola et al., 1996), and treatment with acids and temperature (Tsai et al., 1996). Recently, it was reported that green tea extract prevented gnotobiotic mice from the E. coli infection (Isogai et al., 1998). We have conducted further investigation regarding the growth inhibitory effect of GTC on various E. coli including the serotype O157:H7. 1. Bacterial strains and culture conditions. The bacterial strains used in this study were E. coli O157:H7 Sakai strain which was isolated from a patient involved in the Sakai-city outbreak during the summer of 1996 (Izumiya et al. 1997), E. coli O157:H7 43895, E. coli O139-CH15, E. coli O55-CH20, K99-B41 and IFO-3545. Bacterial strains were transferred from stock cultures by inoculating a loopful of each in trypticase soy broth (TSB) and incubated at 37 ˚C for 24 h. Bacteria were serially transferred to culture for an additional 24 h. Bacteria were collected by centrifugation at 12,000 rpm x 10 min at 4˚C. The cell pellet was then washed with 0.01M phosphate-buffer saline (PBS) (pH 7.2) and resuspended in the same buffer. The concentration of cells was then adjusted to 104 cells/ml. The MIC of GTC against E. coli was measured by the method described in previous sections. 2. Effects on the growth-multiplication. A volume of 0.5 ml cell suspension (104 CFU/ml) was added to 4.5 ml PBS (0.01M) solution or Muller Hilton medium, incubated at 37 ˚C for 0, 2, 4, 6 and 24 h, with or without GTC at various concentrations from 0 to 1000 µg/ml. After incubation, 0.5 ml of bacterial suspension was plated on TS agar medium, incubated at 37 ˚C for 24 h, and the colony counts were performed for viable cells. The MIC of GTC against various strains of E. coli were determined (TABLE 3). GTC has completely inhibited the growth of two strains of E. coli O157:H7 at the concentration of 250 µg/ml, and at 500 or 750 µg/ml against other strains of E. coli. These data suggest that, E. coli O157:H7 was more susceptible to GTC than the other strains of E. coli. The inhibitory effects of GTC against E. coli O157:H7 Sakai strain (FIGURE 6A) and E. coli IFO-3545 (FIGURE 6B) incubated in PBS at 37 ˚C for various time periods was studied. GTC inhibited the growth of both E. coli strains, and the inhibition was increased in a dose-dependent manner with the GTC concentration. The growth of bacteria was completely inhibited by in the buffer solution containing 1,000 µg/ml of GTC for 6 h or at > 200 µg/ml concentration after 24 h incubation. The effect of GTC in Muller Hilton medium on the growth of E.coli was tested. The survival of E. coli IFO-3545 in culture medium after 24 hr incubation was not affected even at the concentration of 1,000 µg/ml of GTC and the viable cell counts of this strain increased from initial count of 105 CFU/ml to 1011 CFU/ml (Figure 6D). On the other hand, GTC at 1000 µg/ml inhibited the growth of E. coli O157:H7 Sakai strain after 24 h of cultivation, and the viable of bacteria decreased from 104 CFU/ml to 0.05) [Redrawn from Marshal & Kim, 1996]. FIGURE 2C. Generation times of aerobic bacteria at 4°C on catfish fillets treated with different levels of sodium acetate. Bars from Left to Right represent levels of 0%, 0.25%, 0.5%, 0.75% and 1.0%, respectively. Means having the same letter are not significantly different (P>0.05) [Redrawn from Kim et al., 1995b].
B. Mechanism of action At equimolar levels, organic acids (weak acids) have greater antimicrobial activity than strong inorganic acids. In addition, the antimicrobial effect of weak acids increases as pH decreases. This implies that the activity of organic acids is directly related to the amount of undissociated molecules (protonated acids), which increase as pH decreases due to increasing amounts of protons (Winslow & Lochridge, 1906; Levine & Fellers, 1940; Ingram et al., 1956; Eklund, 1989; Brown & Booth, 1991; Ray & Sandine, 1992). When acetic acid is dissolved in solution, it dissociates to release free protons, which decrease solution pH. The increased number of protons on the outer surfaces of microorganisms can disrupt membrane function by denaturing enzymes and by altering permeability leading to membrane destabilization (Booth, 1985; Cassio et al., 1987; Ray & Sandine, 1992; Casal et al., 1998). Undissociated acetic acid can also traverse the lipid
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bilayer of bacteria and yeasts and release protons into the cytoplasm (Young & Foegeding, 1993; Casal et al., 1998; Guldfeldt & Arneborg, 1998). Excess intracellular protons can acidify the cytoplasm and cause protein denaturation and energy loss due to activation of ATP-dependant proton pumps located in the cell membrane (Booth, 1985; Pampulha & Loureiro-Dias, 1989; Ray & Sandine, 1992). Because ATP is needed for active transport of nutrients across membranes, cell starvation also can occur due to acetic acid exposure (Ray & Sandine, 1992). Furthermore, the data suggests that bacterial ribosomes are target sites for antimicrobial action of acids (Zayaitz & Ledford, 1985). Thus, it is generally thought that the activity of acetic acid is due to the action of both undissociated and dissociated molecules. When pH is high, the amount of undissociated molecules will be relatively small, which suggests that acetic acid can possibly cause extracellular damage around neutral pH. In contrast, at low pH the amount of protons is higher and the amount of undissociated acetic acid is higher, which results in significantly more internal and external cell damage. This damage can be caused by protons, undissociated molecules, and by acetic acid anions (Ray & Sandine, 1992). The damage caused may be permanent leading to cell death (bactericidal) or may be transient leading to cell injury that either prevents cell multiplication until repair or dramatically slows the rate of cell multiplication (bacteriostatic) (Foster & Hall, 1990). FIGURE 2C shows the increase in generation time (reduction in growth rates) of aerobic spoilage bacteria on catfish exposed to sublethal concentrations of sodium acetate (Kim et al., 1995b). Physiological responses of certain microorganisms to varying concentrations of acetic acid have been investigated (Huang et al., 1986; Diez-Gonzalez & Russell, 1997). At bacteriostatic concentrations of acetic acid or sodium acetate, sublethal injury has been observed in Escherichia coli (Roth & Keenan, 1971; Przybylski & Witter, 1979; Buchanan & Edelson, 1999), Salmonella bareilly (Blankenship, 1981), and Listeria monocytogenes (Ahamed & Marth, 1990). For Clostridium acetobutylicum at pH 4.5, Huang et al. (1986) observed an intracellular concentration of acetic acid that was 13-fold higher than extracellular concentration. This high acid concentration intracellularly resulted in lower cytoplasm pH. Differences in regulation of metabolic processes occurring in response to increases in acetic acid concentration have been reported (Diez-Gonzalez & Russell, 1997; Ita & Hutkins, 1991). Ita & Hutkins (1991) compared intracellular pH effects of acetic, lactic, citric, and hydrochloric acids on L. monocytogenes. In their study, lactic and citric acids reduced intracellular pH more than acetic acid. In contrast, Young & Foegeding (1993) found that acetic acid lowered internal pH of L. monocytogenes more than lactic or citric acids. In both studies, acetic acid reduced numbers of L. monocytogenes more effectively than the other acids tested. In a study comparing responses of nonpathogenic E. coli K-12 to pathogenic E. coli O157:H7, intracellular pH was lower for E. coli O157:H7 as was the observed extracellular to intracellular pH difference, reportedly due to increased lactate production (Diez-Gonzalez & Russell, 1997). The presence of alternative modes of pH regulation in E. coli O157:H7 compared to E. coli K-12 represents an adaptive strategy supporting concerns about the pathogenic strain’s ability to persist in certain foods and cause illness following their consumption. Fermentation acidresistance in bacteria has been characterized by the ability to generate ATP, grow, and/or
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maintain a low pH membrane gradient under conditions generally bacteriostatic (Russell & Diez-Gonzalez, 1998). C. Survival of microorganisms exposed to acetic acid Many studies have demonstrated the ability of acetic acid to inhibit a variety of microorganisms (Osterling & Lindgren, 1993). For example, growth of the peptic ulcer causing bacterium Helicobacter pylori was inhibited by acetic acid (above 0.2 mol/L) and by sodium acetate (above 2.5 mol/L) (Midolo et al., 1995). Chung and Goepfert (1970) demonstrated that acetic acid was more lethal than lactic acid to Salmonella spp. Similarly, acetic acid had greater activity against Yersinia enterocolitica during low temperature incubation than lactic, citric, or sulfuric acids (Brackett, 1987; Little et al., 1992). Ryu et al. (1999) showed that acetic acid inhibited E. coli O157:H7 better than lactic, malic, or citric acids. Vegetative cells of Bacillus cereus were inhibited more by acetic acid than by formic acid (Wong & Chen, 1988). In contrast, spore germination of B. cereus was inhibited more by formic acid than acetic acid (Wong & Chen, 1988). Other bacilli (B. subtilis and B. licheniformis) known to cause rope spoilage of bread were inhibited by 0.1% acetic acid (Rosenquist & Hansen, 1998). Bacteriostatic activity of acetic acid against L. monocytogenes was reported at 0.2% and bactericidal activity was found at concentrations exceeding >0.3% (Ahamad & Marth, 1987; Farber et al., 1989). Activity against this pathogen increased as incubation temperature increased (Ahamad & Marth, 1987, Sorrells et al., 1989). In addition, the effects of pH and salt on sodium acetate inhibition of L. monocytogenes has been reported (Nerbrink et al., 1999). Greater than 5 log reductions in the numbers of Campylobacter jejuni could be achieved with a 2.5 minute exposure to 1% acetic acid at 50˚C (Stern et al., 1985). One and two log reductions were observed in the population of Staphylococcus aureus inoculated into milk acidified to pH 5.2 and 5.0 with acetic acid, respectively (Minor & Marth, 1970). Growth and aflatoxin production by Aspergillus parasiticus were reduced as concentration of acetic acid increased from 0 to 0.75%, with activity of acetic acid increasing as pH decreased (Rusul et al., 1987). Implication of acidic foods like apple cider (Besser et al., 1993) and apple juice (Steele et al., 1982) as transmission vehicles in outbreaks of E. coli O157:H7 infections, has shifted research focus on acetic acid. Emphasis on the acid-tolerance of E. coli O157:H7 has generated numerous reports investigating growth and survival of this bacterium in foods typically acidified with acetic acid, such as apple cider (Zhao et al., 1993; Miller & Kaspar, 1994; Semanchek & Golden, 1996), mayonnaise (Weagant et al., 1994; Zhao & Doyle, 1994; Erickson et al., 1995; Hathcox et al., 1995; Raghubeer et al, 1995), and even vinegar (Tsujihata et al., 1998). Acid tolerance has been determined to be a characteristic trait of E. coli O157:H7 rather than a response (Leyer et al., 1995). This trait is enhanced at refrigeration temperatures (Miller & Kaspar, 1994). High survival rates have been reported for E. coli O157:H7 during refrigerated storage of apple ciders containing preservatives (Miller & Kaspar, 1994). Also, Salmonella typhimurium, S. aureus, and E. coli O157:H7 survival in mayonnaise and mayonnaise-based products has been investigated (Wethington & Fabian, 1950; Doyle et al., 1982; Gomez-Lucia et al., 1987; Weagant et al., 1994; Zhao & Doyle, 1994; Raghubeer et al., 1995). Mayonnaise acidified to pH 3 logs) in numbers of E. coli O157:H7 on cutting boards after surface treatment with vinegar solutions (1 to 2% acetic acid) containing added salt (3 to 7%). B. Decontamination of meats Effectiveness of acetic acid for decontamination of beef and pork carcasses has been reviewed (Dickson & Anderson, 1992; Frederick, 1994; Siragusa, 1995; Bolder, 1997; Smulders & Greer, 1998). The effectiveness of acetic acid as a carcass decontaminating treatment depends on a number of factors. In general, the efficacy of acetic acid increases with increasing treatment temperature, increasing acid concentration, and decreasing level of carcass contamination (Greer & Dilts, 1992). Meat-associated pathogens, such as Y. enterocolitica, L. monocytogenes, S. typhimurium, E. coli, Campylobacter jejuni, and S. aureus, are more resistant to acetic acid than are spoilers, such as Pseudomonas fragi and Brochothrix thermosphacta (Greer & Dilts, 1992).
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Of the many carcass decontamination procedures, treatment with acetic acid has been shown to be the best chemical treatment over steam, hot water, hypochlorite, hydrogen peroxide, or trisodium phosphate (Anderson et al., 1979; Cabedo et al., 1996). Acetic acid treated beef plates had at least a 16 day shelf-life extension compared to untreated plates as determined by total plate counts (Anderson et al., 1979) presumably due to the 1.5 log decrease in total microbial counts achieved with 3% acetic acid treatment (Anderson et al., 1980). Beef carcasses spray washed with 1% acetic acid and then stored under vacuum had lower aerobic plate counts than untreated samples, with lactobacilli predominating (Hamby et al., 1987). Pork products treated with 2-3% acetic acid and vacuum packaged had lower aerobic, anaerobic, psychrotrophic, lactic acid, and Enterobacteriaceae bacterial counts, which yielded products having much longer refrigerated shelf-life (Mendonca et al., 1989; Cacciarelli et al., 1983). Hot (52˚C) acetic acid (1.5%) carcass wash solution was more effective in reducing microbial counts than was cooler solution (14.4˚C) (Anderson et al., 1987). Similar findings were found using 55˚C acetic acid dips compared with 25˚C dips to decontaminate lamb carcasses (Anderson et al., 1988). Increasing temperature of dip solution to 70˚C allowed for substantial reduction in total aerobic plate counts, Enterobacteriaceae counts, E. coli counts, and Salmonella counts even with low (1%) acetic acid concentrations (Anderson & Marshall, 1989). Beef carcasses contaminated with feces were effectively decontaminated by washing followed by organic acid treatment than by washing alone or trimming (Hardin et al., 1995). Aerobic plate counts, coliform counts, and the incidence of Salmonella contamination all decreased on pork cheek meat treated with 2% acetic acid (Frederick et al., 1994). Dickson (1992) demonstrated that 65% of a S. typhimurium population was sublethally injured on lean and fat tissues of beef when treated with 2% acetic acid. When acetic acid was combined with calcium alginate gel and applied to beef tissue, counts of S. typhimurium, L. monocytogenes, and E. coli O157:H7 were generally reduced to a similar level as seen with acetic acid alone (Siragusa & Dickson, 1993). A 2% acetic acid spray wash was superior to spray washing with 0.003% chlorine, 5% hydrogen peroxide, or 12% trisodium phosphate in reducing the number of aerobic plate counts on lamb carcasses (Kochevar et al., 1997). Effectiveness of 2% acetic acid can be increased when carcass surfaces are dried or treated with 20% NaCl to cause osmotic stress of bacteria (Dickson, 1990). A combination of 15 ml/L acetic acid dip (55˚C) for 10 sec with vacuum packaging significantly increased refrigerated shelf-life of pork (Shay & Egan, 1986). A further refinement of acetic acid carcass washing has shown dramatic reductions in total counts and E. coli counts when carcasses were washed twice with 2% acetic acid during processing (Graves Delmore et al., 1998). In this study, carcasses were washed pre-evisceration and after final carcass fabrication. Count reductions achieved were 2.9 and 4.3 logs for high inoculum levels of aerobes and E. coli, respectively. It has been shown that bacterial reduction of carcasses by acetic acid is better on adipose tissue than on lean tissue (Cutter & Siragusa, 1994). Saponins (plant-derived triterpenoid glycosides) added as foaming agents to acetic acid spray washes did not increase effectiveness of acetic acid in reducing the levels of pathogens and spoilers on beef (Cutter, 1999). Dorsa et al. (1997; 1998a; 1998b) assessed effectiveness of several beef carcass wash treatments (2% lactic acid, 2% acetic acid, 12% trisodium phosphate, water at 78˚C, water at 32˚C, and untreated as experimental control) for beef subprimals and ground beef
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control or elimination of S. typhimurium, L. monocytogenes, E. coli O157:H7, or Clostridium sporogenes. Their work demonstrated that acetic acid offered residual antimicrobial activity on subprimals during vacuum packaged chill storage (Dorsa et al., 1998a). For the ground beef studies (Dorsa et al., 1998b), treated beef carcass tissue was inoculated with low or high numbers of pathogens, and microbiological sampling was performed i) less than 30 minutes after treatment and ii) after 24 h storage at 4˚C for treated carcasses, iii) immediately following processing to ground beef, and iv) after storage at 12˚C for 3 days or 4˚C for 21 days. Surface pH of acetic acid-treated carcasses increased from 4.3 (following acetic acid exposure) to 4.9 after 24 h at 4˚C. Following processing to ground beef, an additional increase to pH 5.7 was reported for acetic acid treatment (Dorsa et al., 1998b). Ground beef processed from carcasses treated with acetic acid, lactic acid, TSP, or hot water (78˚C) had lower numbers of recovered E. coli O157:H7 (high inoculum) than did ground beef made from carcasses treated with water (32˚C) or left untreated (as controls). For samples inoculated with low levels of E. coli O157:H7, only acetic acid treatment resulted in significantly lower numbers of E. coli O157:H7 following storage at 12˚C for 3 days. In general, carcass wash treatments were effective in reducing numbers of pathogens (low level inoculum) subsequently recovered in ground beef after storage for 3 days at 12˚C (Dorsa et al., 1998b). Additionally, acetic acid carcass treatment reduced total aerobic and pseudomonad counts on ground beef stored for 3 days at 12˚C (Dorsa et al., 1998b) compared to controls. No difference was reported for these counts following refrigeration storage (4˚C) for 21 days (Dorsa et al., 1998b); however, the authors reported a trend of gradually decreasing numbers of pseudomonads and total aerobic bacterial counts for ground beef processed from acetic acid-washed carcasses. The primary approach of Dorsa et al. (1998a; 1998b) was microbial profiling to test whether or not reduction of overall bacterial numbers resulted with concurrent increases in numbers of pathogens due to lack of competition. Therefore, the main conclusion was that antimicrobial treatments, while not dramatically reducing total microbial counts, were effective for pathogen control, and initial reductions of total microbial numbers did not result in increases in pathogen levels (Dorsa et al., 1998a; 1998b). Others have found that acetic acid treatment of low count carcasses has little benefit. For example, Ockerman et al. (1974) found small reductions in microbial counts on lamb carcasses sprayed with 6% acetic acid. Beef carcasses treated with 5% acetic acid showed less than a 1 log reduction in inoculated E. coli O157:H7 (Delazari et al., 1998). Likewise, Brackett et al. (1994) showed that 1.5% acetic acid was not effective in reducing the levels of E. coli O157:H7 on beef. In addition, Conner et al., (1997) found that 24% acetic sprays of beef trim destined for ground beef manufacture had little impact on the survival of inoculated E. coli O157:H7 and L. monocytogenes. These studies differed from those described previously because the beef chosen for use was post-chill retail cuts rather than pre-chill carcasses. Fu et al. (1994) showed that pork carcasses sprayed with 1.5% acetic acid had lower coliform counts initially but when carcasses were processed into loins this effect was minimal during storage. Likewise, in a commercial beef slaughter plant, dilute acetic acid spray was ineffective in reducing microbial counts of low count carcasses (Avens et al., 1996). The latter experiment failed to adequately describe the concentration of acetic acid used. Thus, given the abundance of evidence showing efficacy of acetic acid as a pre-chill carcass decontaminating agent, use of acetic acid would be best in this circumstance. Use on post-chill beef cuts seems to render acetic acid less potent. © 2000 by CRC Press LLC
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Unfortunately, direct acetic acid treatment of meat pieces can lead to discoloration (Kotula & Thelappurate, 1994) and off flavors (Bell et al., 1986), thus making acetic acid decontamination treatments only valid for carcass decontamination. Although treatment of animal carcasses and consumer cuts with acetic acid can reduce microbial loads, there remains the question of whether such treatments yield marketable products. Kotula & Thelappurate (1994) showed that sensory panelists were generally unable to differentiate 1.2% acetic acid treated retail beef cuts from those that were untreated. C. Decontamination of poultry As with treatment conditions described with meats, acetic acid can also increase the shelf-life of poultry by inhibiting growth of spoilage bacteria (Mountney & O’Malley, 1965). Acetic acid can aid in controlling Salmonella cross-contamination from scald tank water to bird carcasses; however, treatment with acetic acid may not result in lower aerobic microbial counts on picked carcasses (Lillard et al., 1987; Dickens & Whittemore, 1994). This suggests that carcass cross-contamination can occur during picking. Others, however, have shown that 1% acetic acid treatment for 30 seconds produced a 0.6 log reduction in total aerobic plate counts (Dickens & Whittemore, 1997) and 0.6% acetic acid treatment for 10 min gave a 0.7 log reduction in Enterobacteriaceae counts (Dickens et al., 1994). Five percent acetic acid was effective in reducing the number of S. typhimurium attached to chicken skin by greater than 2 logs in both chiller and scalder applications (Tamblyn et al., 1997). A 0.8 log reduction in the numbers of C. jejuni was achieved with a 0.5% acetic acid immersion at 50°C for 90 seconds (Stern et al., 1985). Addition of acetic acid to chill tank water or scald tank water may be useful to control pathogens during immersion processing and might reduce the rate of carcass cross-contamination. Indeed, Okrend et al. (1986) found dramatic reductions in D52 of S. typhimurium, Salmonella newport, and C. jejuni when scald water contained as little as 0.1% acetic acid. Increasing acetic acid concentration to 1% caused immediate bacterial death at 52 °C. For control of L. monocytogenes growth on vacuum packaged turkey bologna, 0.5% sodium acetate proved slightly superior to 1.0% sodium bicarbonate, 2.0% sodium lactate, or 0.26% potassium sorbate as formulation additives (Wederquist et al., 1994). Even though microbial count reductions on chickens following immersion in acetic acid solutions largely have not been significant, reported decreases in numbers of Enterobacteriaceae and/or Salmonella spp. recovered from immersion solution samples have potentially significant ramifications in cross-contamination control. Evaluation of poultry processing steps in order to identify contamination points for Salmonella or factors influencing pathogen incidence from fresh poultry products have resulted in development and evaluation of various treatments for pathogen control (Lillard, 1990). D. Decontamination of seafoods Catfish fillet aerobic plate counts were reduced by treatment with sodium acetate (FIGURE 2A) (Kim et al., 1995b). This resultant inhibition of microbial spoilers gave a 6 day shelf-life increase of fillets during refrigerated storage presumably due to slowing the growth rate of survivors (FIGURE 2C). Combining 0.7% sodium acetate with 0.4% monopotassium phosphate gave microbial growth rate retardation (FIGURE 5B) that was similar to that seen with use of 1% sodium acetate alone (FIGURE 2C) (Kim et al., 1995b). Sensory panelists found that fillets treated with the combined chemicals were preferred over untreated controls during storage (Kim et al., 1995b). It was concluded that most of © 2000 by CRC Press LLC
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FIGURE 5A. Aerobic plate counts of catfish fillets treated with Bifidobacterium infantis culture and sodium acetate, either alone or combined, during storage at 4°C. Control (!), 2.5% B. infantis (❒), 0.5% sodium acetate (❍), and a combination of both ($). [Redrawn from Kim et al., 1995a]. FIGURE 5B. Generation times of aerobic bacteria at 4°C on catfish fillets treated with combinations of sodium acetate (0.5%) and different concentrations of monopotassium phosphate. Bars from Left to Right represent control, 0.1%, 0.2%, 0.3% and 0.4% monopotassium phosphate, respectively, in combination with 0.5% sodium acetate. [Redrawn from Kim et al., 1995b]. FIGURE 5C. Generation times of aerobic bacteria at 4°C on catfish fillets treated with different concentrations of acetic acid or lactic acid. Bars from Left to Right represent acid concentrations, 0%, 1%, 2%, 3% and 4%, respectively. [Redrawn from Marshal & Kim, 1996].
the antimicrobial effect was associated with sodium acetate and the combined effect with monopotassium phosphate was additive. Growth of Gram negative bacteria was prevented for 6 days on catfish fillets treated with 1% sodium acetate (Kim & Hearnsberger, 1994). In this study sodium acetate was also combined with 0.25% potassium sorbate and 2.5% Lactococcus lactis culture to test for interactions between the treatments. Results demonstrated that antimicrobial activity resided primarily with acetate. The addition of sorbate or lactic culture had little impact on inhibiting Gram negative bacteria. In a similar study, Kim et al. (1995a) showed that a combination of 0.5% sodium acetate and a 2.5% culture of Bifidobacterium infantis gave greater inhibition of aerobic microorganisms than did either acetate or culture alone (FIGURE 5A). Thus, the interaction between © 2000 by CRC Press LLC
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FIGURE 6. 2% acid-treated catfish fillets (Cf) during storage at 4 C. Unrinsed ( !), rinsed ( ) or treated with acetic (A: "), citric (C: ❒), hydrochloric (H: --), lactic (L: $), malic (M: ❍), and tartaric (T: ✶) acids. FIGURE 6A. Change in aerobic plate counts; FIGURE 6B. Change in coliform counts; FIGURE 6C. Change in Listeria monocytogenes counts; FIGURE 6D. Composite representation of dip solution pH (solid bar), catfish fillet surface pH (open bar), and pKa (") of treatment acids. [Redrawn from Bal’a & Marshall, 1998].
acetate and B. infantis culture was deemed an additive response. Acetate treatment, whether alone or combined with culture, increased refrigerated shelf-life of fillets by 3 days (Kim et al., 1995a). Like many previous studies comparing the activity of acetic acid with other acids, Marshall & Kim (1996) demonstrated that acetic acid slowed the rate of growth of aerobic spoilage bacteria more than did lactic acid (FIGURE 5C). More recently, Bal’a and Marshall (1998) demonstrated that 2% acetic acid had greatest inhibitory ability towards catfish fillet aerobic (FIGURE 6A), coliform (FIGURE 6B), and L. monocytogenes (FIGURE 6C) bacteria compared to 2% concentrations of citric, lactic, malic, tartaric, or hydrochloric acids. They also demonstrated that among the acids tested, acetic acidtreated fillets had the highest surface pH (FIGURE 6D). Thus, the greater activity of acetic acid was not due to its ability to reduce surface pH lower than the other acids. These
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results were subsequently confirmed by Fernandes et al. (1998). Marshall & Kim (1996) demonstrated that catfish fillets treated with greater than 2% acetic acid were objectionable to sensory panelists in terms of off-color and off-odor problems. Crabmeat contaminated with L. monocytogenes showed 0.8 log or 2.0 log reductions in counts after washing with 4 M sodium acetate or 2 M sodium diacetate solutions for 1 minute (Degnan et al., 1994). Acetic acid was superior to formaline and orthrophosphoric, formic, tartaric, citric, hydrochloric, and sulfuric acids in preserving mackerel fish destined for fish meal production (Borquez et al., 1994). In addition, processing performance of acetic acid treated mackerel during fish-meal production was superior to untreated controls (Borquez & Gonzalez, 1994). Treatment of whole and peeled shrimp with sodium acetate improved initial microbiological quality and extended shelf-life (Zhuang et al., 1996; Al-Dagal & Bazaraa, 1999). Sodium acetate was superior to treatment with potassium sorbate, sodium lactate, trisodium citrate, or bifidobacteria culture. E. Decontamination of produce and grains Fruit decay could be prevented by fumigation with >2 mg acetic acid vapor per liter of air (Sholberg & Gaunce, 1995). Apples and pears inoculated with the molds Botrytis cinerea and Penicillium expansum failed to decay. Similarly, tomatoes, grapes, and kiwifruit contaminated with B. cinerea and oranges contaminated with Penicillium italicum failed to decay when fumigated with acetic acid at 5˚C. Greater activity of acetic acid was obtained at high relative humidity (98%) (Sholberg & Gaunce, 1995). Table grapes fumigated with 0.27% acetic acid yielded results similar to fumigation with sulfur dioxide, with effective control of both Botrytis and Penicillium decay during refrigerated storage (Sholberg et al., 1996). Decay of peaches by Monilinia fructicola and Rhizopus stolonifer could be prevented by fumigation with 1.4 to 2.7 mg/L acetic acid (Sholberg & Gaunce, 1996a). Additionally, Alternaria decay of cherries and brown rot (M. fructicola) of apricots could be reduced with acetic acid fumigation (Sholberg & Gaunce, 1996a). An additional study has shown that nectarines, oranges, lemons, and grapefruits fumigated with 1.9 µl/L acetic acid could reduce decay from 98% to 16% for nectarines and from 86% to 11% for citrus during storage at 20˚C (Sholberg, 1998). Acetic acid fumigation combined with low carbon dioxide modified atmosphere packaging increased strawberry shelf-life 2-3 fold (Moyles et al., 1996). Fumigated strawberries were free of decay for 14 days at 5˚C while untreated strawberries had 89% rotted fruits by this time. Proliferation of aflatoxigenic Aspergillus flavus in high moisture rape, rice, and wheat grains could be controlled by fumigation with acetic acid (Sholberg & Gaunce, 1996b). A fumigation treatment with 0.50 ml acetic acid/100 g cabbage resulted in undetectable levels of microorganisms on prepared coleslaw after 22 days of storage at 5˚C (Delaquis et al., 1997). This fumigation treatment of shredded cabbage prior to processing to coleslaw proved to reduce the numbers of spoilage bacteria and extend refrigerated shelf-life. In contrast, numbers of L. monocytogenes on cabbage and lettuce could not be effectively reduced by a 10 min exposure to 1% acetic acid (Zhang & Farber, 1996). Entani et al. (1997) reported effective reductions (>3 logs) in numbers of E. coli O157:H7 on cabbage and cucumbers after surface treatment with vinegar solutions (1 to 2% acetic acid) containing added salt (3 to 7%). Mung bean seeds used to produce bean sprouts were fumigated with 242 µl acetic acid per liter of air for 12 hours at 45˚C
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FIGURE 7. Generation times of aerobic bacteria at 4°C on catfish fillets treated with sodium acetate and Bifidobacterium infantis. Bars from Left to Right represent control, 2.5% B. infantis, 0.5% sodium acetate and a combination of both, respectively. Means having the same letter are not significantly different (P>0.05) [Redrawn from Kim et al., 1995a].
(Delaquis et al., 1999). This treatment yielded 5, 6, and 4 log reductions in contaminating S. typhimurium, E. coli O157:H7, and L. monocytogenes without adversely affecting sprouting performance of the seeds. F. Natural preservation systems Natural preservation systems for food have incorporated cultures of lactic acid bacteria, bifidobacteria, and propionic bacteria (Kim & Hearnsberger, 1994; Kim et al., 1995a). For example, bifidobacteria culture combined with sodium acetate slowed the rate of growth of aerobic spoilage bacteria on catfish fillets greater than either treatment alone (FIGURE 7). Use of desirable microorganisms in natural systems-approaches works because they form and/or accumulate starter culture-derived compounds, such as lactic, acetic, or propionic acids (Ray & Sandine, 1992), nisin (Ray, 1992a), and/or acetaldehyde (Ray, 1992b). These compounds individually or combined have antimicrobial activities that can extend shelf-life of certain food products or inhibit foodborne pathogens (Daeschel, 1989; Ray, 1992a). Shelf-life extension of various products has been approached by incorporating bacteriocins of lactic acid bacteria (Davies et al., 1997). The effects of combining acetic acid with bacteriocins or other naturally occurring antimicrobial compounds, such as chitosan, protamine, lysozyme, and lactoferrin have not been reported.
VI. REGULATORY STATUS Acetic acid, used and label-listed generally as vinegar, has been employed as a flavoring ingredient but also has functioned primarily as an acidulant or preservative in foods (Gardner, 1968; Stroup et al., 1985). Excluding vinegar, the foremost food types important when considering acetic acid are mayonnaise, salad dressings, ketchups/catsups, sauces or condiments, and pickles and relishes (Fabian & Wadsworth, 1939; Gardner, 1968; Kabara & Eklund, 1991; Davidson, 1997). Other foods containing acetic © 2000 by CRC Press LLC
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acid include cheeses and non-dairy equivalents, baked products, oils, gravies, and meat products (Davidson, 1997). Acetic acid is the preferred acidulant used to make direct set soft-style cheeses such as Queso Blanco (Farkye et al, 1995). Acetic acid is frequently used to prevent ropy spoilage of breads (Rosenquist & Hansen, 1998); however, levels used must not inhibit fermentation ability of the leavening yeast Saccharomyces cerevisiae (Phowchinda et al., 1995). Principle U.S. regulations for use of acetic acid and its salts are found in the Code of Federal Regulations (CFR), Title 21, Volume 3, Parts 170-199. In addition, these food ingredients meet specifications outlined in Food Chemicals Codex. Defined uses of acetic acid are as a pickling and curing agent (21 CFR 184.1005 Sec. 170.3(o)(5)), flavor enhancer (Sec. 170.3(o)(11)), flavoring agent and adjuvant (Sec. 170.3(o)(12)), pH control agent (Sec. 170.3(o)(23)), and carrier solvent (Sec. 170.3(o)(27)). It may be used at levels not exceeding recommendations outlined for current good manufacturing practices (Sec. 184.1(b)(1)). For example, there is a 0.25% limit in baked goods (Sec. 170.3(n)(1)), 0.8% in cheese (Sec. 170.3(n)(5)) and dairy product analogs (Sec. 170.3(n)(10)), 0.5% in chewing gum (Sec. 170.3(n)(6)), 9.0% in condiments and relishes (Sec. 170.3(n)(8)), 0.5% in fats and oils (Sec. 170.3(n)(12)), 3.0% in gravies and sauces (Sec. 170.3(n)(24)), 0.6% in meat products (Sec. 170.3(n)(29)), and 0.15% or less in other food product categories. Calcium acetate is used as a firming agent (21 CFR 184.1185 Sec. 170.3(o)(10)), pH control agent (Sec. 170.3(o)(23)), processing aid (Sec. 170.3(o)(24)), sequestrant (Sec. 170.3(o)(26)), stabilizer and thickener (Sec. 170.3(o)(28)), and texturizer (Sec. 170.3(o)(32)). Usage limits for this compound are 0.2% in baked goods (Sec. 170.3(n)(1)), 0.02% in cheese (Sec. 170.3(n)(5)), 0.2% in gelatins, puddings, and fillings (Sec. 170.3(n)(22)), 0.15% in sweet sauces, toppings, and syrups (Sec. 170.3(n)(43)), and 0.0001% for all other food categories. Sodium acetate is used as a flavoring agent and adjuvant (21 CFR 184.1721 Sec. 170.3(o)(12)) and as a pH control agent (Sec. 170.3(o)(23)). It may be used at levels not exceeding 0.007% in breakfast cereals (Sec. 170.3(n)(4)), 0.5% in fats and oils (Sec. 170.3(n)(12)), 0.6% in grain products and pastas (Sec. 170.3(n)(23)) and snack foods (Sec. 170.3(n)(37)), 0.15% in hard candy (Sec. 170.3(n)(25)), 0.12% in jams and jellies (Sec. 170.3(n)(28)) and meat products (Sec. 170.3(n)(29)), 0.2% in soft candy (Sec. 170.3(n)(38)), 0.05% in soups and soup mixes (Sec. 170.3(n)(40)) and sweet sauces (Sec. 170.3(n)(43)). Sodium diacetate is used as an antimicrobial agent (21 CFR 184.1754 Sec. 170.3(o)(2)), flavoring agent and adjuvant (Sec. 170.3(o)(12)), and pH control agent (Sec. 170.3(o)(23)). Maximum usage levels are 0.4% in baked goods (Sec. 170.3(n)(1)), 0.1% in fats and oils (Sec. 170.3(n)(12)), meat products (Sec. 170.3(n)(29)), and soft candy (Sec. 170.3(n)(38)), 0.25% in gravies and sauces (Sec. 170.3(n)(24)), and 0.05% in snack foods (Sec. 170.3(n)(37)) and soups and soup mixes (Sec. 170.3(n)(40)).
VII. SUMMARY Acetic acid and its GRAS salts have a long history of functional use in foods. The ability to lower pH with acetic acid or vinegar provides pickled foods with unsurpassed keeping quality, flavor, and safety. Aside from this traditional use, acetic acid use as a
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decontaminating agent of fresh and minimally processed foods remains under exploited. Few other naturally occurring antimicrobial agents have such a wide spectrum of activity. Newer uses of acetic acid will likely be discovered. Food processors should find acetic acid a desirable functional ingredient or processing aid because of its wide availability, low cost, consumer acceptance, and clean label requirements.
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100. Hamby, P.L., Savell, J.W., Acuff, G.R., Vanderzant, C., and Cross, H.R. 1987. Spray-chilling and carcass decontamination systems using lactic acid and acetic acid. Meat Sci. 21: 1-14. 101. Hardin, M.D., Acuff, G.R., Lucia, L.M., Oman, J.S., and Savell, J.W. 1995. Comparison of methods for decontamination from beef carcass surfaces. J. Food Prot. 58: 368-374. 102. Hartwig, P. and McDaniel, M. R. 1995. Flavor characteristics of lactic, malic, citric, and acetic acids at various pH levels. J. Food Sci. 60: 384-388. 103. Hathcox, A.L., Beuchat, L.R., and Doyle, M.P. 1995. Death of enterohemorrhagic Escherichia coli O157:H7 in real mayonnaise and reduced-calorie mayonnaise dressings as influenced by initial population and storage temperature. Appl. Environ. Microbiol. 61: 4172-4177. 104. Hentges, D.J. 1967. Influence of pH on the inhibitory activity of formic and acetic acids for Shigella. J. Bacteriol. 93: 956-958. 105. Huang, L., Forsberg, C.W., and Gibbins, L.N. 1986. Influence of external pH and fermentation products of Clostridium acetobutylicum intracellular pH and cellular distribution of fermentation products. Appl. Environ. Microbiol. 51: 1230-1234. 106. Ingram, M., Ottoway, F.J.H., and Coppock, J.B.M. 1956. The preservative action of acid substances in food. Chem. Ind. (London) 42: 1154-163. 107. Ita, P.S. and Hutkins, R.W. 1991. Intracellular pH and survival of Listeria monocytogenes Scott A in tryptic soy broth containing acetic, lactic, citric, and hydrochloric acids. J. Food Prot. 54: 15-19. 108. Ito, K.A., Chen, J.K., Lerke, P.A., Seeger, M.L., and Unverferth, J.A. 1976. Effect of acid and salt concentration in fresh-pack pickles on the growth of Clostridium botulinum spores. Appl. Environ. Microbiol. 32: 121-124. 109. Ito, T., Sota, H., Honda, H., Shimizu, K., and Kobayashi, T. 1991. Efficient acetic acid production by repeated fed-batch fermentation using two fermentors. Appl. Microbiol. Biotech. 36: 295-299. 110. Kabara, J.J. and Eklund, T. 1991. Organic acids and esters. In Food Preservatives, ed. N.J. Russell and G.W. Gould, pp. 44-71. Glasgow: Blackie and Son Ltd. 111. Karl, H., Roepstorff, A., Huss, H.H., and Bloemsma, B. 1994. Survival of Anisakis larvae in marinated herring fillets. Int. J. Food Sci. Technol. 29: 661-670. 112. Kim, C.R. and Hearnsberger, J.O. 1994. Gram negative bacteria inhibition by lactic acid culture and food preservatives on catfish fillets during refrigerated storage. J. Food Sci. 59: 513-516. 113. Kim, C.R., Hearnsberger, J.O., Vickery, A.P., White, C.H., and Marshall, D.L. 1995a. Sodium acetate and bifidobacteria increase shelf-life of refrigerated catfish fillets. J. Food Sci. 60: 25-27. 114. Kim, C.R., Hearnsberger, J.O., Vickery, A.P., White, C.H., and Marshall, D.L. 1995b. Extending shelf life of refrigerated catfish fillets using sodium acetate and monopotassium phosphate. J. Food Prot. 58: 644647. 115. Kochevar, S.L., Sofos, J.N., LeValley, S.B., and Smith, G.C. 1997. Effect of water temperature, pressure and chemical solution on removal of fecal material and bacteria from lamb adipose tissue by spray-washing. Meat Sci. 45: 377-388. 116. Kotula, K.L. and Thelappurate, R. 1994. Microbiological and sensory attributes of retail cuts of beef treated with acetic and lactic acid solutions. J. Food Prot. 57: 665-670. 117. Krueger, D.A. 1992. Stable carbon isotope ratio method for detection of corn-derived acetic acid in apple cider vinegar: collaborative study. J. AOAC Int. 74: 725-728. 118. Kurtzman, C.P., Hesseltine, C.W., and Rogers, R. 1971. Microbiological spoilage of mayonnaise and salad dressing. Appl. Microbiol. 21: 870-874. 119. Lazaro, M.J., Carbonell, E., Aristoy, M.C., Safon, J., and Rodrigo, M. 1989. Liquid chromatographic determination of acids and sugars in homolactic cucumber fermentations. J. Assoc. Off. Anal. Chem. 72: 52-55. 120. Lee, I.S., Lin, J., Hall, H.K., Bearson, B., and Foster, J.W. 1995. The stationary-phase sigma factor (RpoS) is required for a sustained acid tolerance response in virulent Salmonella typhimurium. Mol. Microbiol. 17: 155-167. 121. Levine, A.S. and Fellers, C.R. 1940. Action of acetic acid on food spoilage microorganisms. J. Bacteriol. 39: 499-515. 122. Leyer, G.J. and Johnson, E.A. 1993. Acid adaptation induces cross-protection against environmental stresses in Salmonella typhimurium. Appl. Environ. Microbiol. 59: 1842-1847. 123. Leyer, G.J., Wang, L.-L., and Johnson, E.A. 1995. Acid adaptation of Escherichia coli O157:H7 increases survival in acidic foods. Appl. Environ. Microbiol. 61: 3752-3755. 124. Lillard, H.S. 1990. The impact of commercial processing procedures on the bacterial contamination and cross-contamination of broiler carcasses. J. Food Prot. 53: 202-204, 207. 125. Lillard, H.S., Blankenship, L.C., Dickens, J.A., Craven, S.E., and Shackelford, A.D. 1987. 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153. Pampulha, M.E. and Loureiro-Dias, M.C. 1989. Combined effect of acetic acid, pH and ethanol on intracellular pH of fermenting yeast. Appl. Microbiol. Biotechnol. 31: 547-550. 154. Pangborn, R.M. 1963. Relative taste intensities of selected sugars and organic acids. J. Food Sci. 28: 726733. 155. Parish, M.E. and Higgins, D.P. 1989. Survival of Listeria monocytogenes in low pH model broth systems. J. Food Prot. 52: 144-147. 156. Park, Y.S., Toda, K., Fukaya, M., Okumura, H., and Kawamura, Y. 1991. Production of a high concentration of acetic acid by Acetobacter aceti using a repeated fed-batch culture with cell recycling. Appl. Microbiol. Biotech. 35: 149-153. 157. Pederson, C.S. 1979. Microbiology of Food Fermentations, 2nd Ed. Westport, CT: AVI Publishing Co. 158. Perales, I. and Garcia, M.I. 1990. The influence of pH and temperature on the behavior of Salmonella enteritidis phage type 4 in homemade mayonnaise. Lett. Appl. Microbiol. 10: 19-22. 159. Phowchinda, O., Delia-Dupuy, M.L., and Strehaiano, P. 1995. Effects of acetic acid on growth and fermentative activity of Saccharomyces cerevisiae. Biotechnol. Lett. 17:237-242. 160. Przybylski, K.S. and Witter, L.D. 1979. Injury and recovery of Escherichia coli after sublethal acidification. Appl. Environ. Microbiol. 37: 261-265. 161. Raghubeer, E.V., Ke, J.S., Campbell, M.L., and Meyer, R.S. 1995. Fate of Escherichia coli O157:H7 and other coliforms in commercial mayonnaise and refrigerated salad dressing. J. Food Prot. 58: 13-18. 162. Ray, B. 1992a. Cells of lactic acid bacteria as food biopreservatives. In Food Biopreservatives of Microbial Origin, ed. B. Ray, pp. 81-101. Boca Raton, FL: CRC Press, Inc. 163. Ray, B. 1992b. Diacetyl of lactic acid bacteria as a food biopreservative. In Food Biopreservatives of Microbial Origin, ed. B. Ray, pp. 137-153. Boca Raton, FL: CRC Press, Inc. 164. Ray, B. and Sandine, W.E. 1992. Acetic, propionic, and lactic acids of starter culture bacteria as biopreservatives. In Food Biopreservatives of Microbial Origin, ed B. Ray, pp. 103-136. Boca Raton, FL: CRC Press, Inc. 165. Rice, A.C. and Pederson, C.S. 1954. Factors influencing growth of Bacillus coagulans in canned tomato juice. II. Acidic constituents of tomato juice and specific organic acids. Food Res. 19: 124-133. 166. Rosenquist, H. and Hansen, A. 1998. The antimicrobial effect of organic acids, sour dough and nisin against Bacillus subtilis and B. licheniformis isolated from wheat bread. J. Appl. Microbiol. 85: 621-631. 167. Roth, L.A. and Keenan, D. 1971. Acid injury of Escherichia coli. Can. J. Microbiol. 17: 1005-1008. 168. Russell, J.B. and Diez-Gonzalez, F. 1998. The effects of fermentation acids on bacterial growth. Adv. Microbiol. Physiol. 39: 205-234. 169. Rusul, G., El-Gazzar, F.E., and Marth, E.H. 1987. Growth and aflatoxin production by Aspergillus parasiticus NRRL 2999 in the presence of acetic or propionic acid and at different initial pH values. J. Food Prot. 50, 909-914. 170. Ryu, J.-H. and Beuchat, L.R. 1998. Influence of acid tolerance responses on survival, growth, and thermal cross-protection of Escherichia coli O157:H7 in acidified media and fruit juices. Int. J. Food Microbiol. 45: 185-193. 171. Ryu, J.-H., Deng, Y., and Beuchat, L.R. 1999. Behavior of acid-adapted and unadapted Escherichia coli O157:H7 when exposed to reduced pH achieved with various organic acids. J. Food Prot. 62: 451-455. 172. Semanchek, J.J. and Golden, D.A. 1996. Survival of Escherichia coli O157:H7 during fermentation of apple cider. J. Food Prot. 59: 1256-1259. 173. Shay, B.J. and Egan, A.F. 1986. Studies of possible techniques for extending the storage life of chilled pork. Food Technol. Aust. 38: 144-146. 174. Sholberg, P.L. 1998. Fumigation of fruit with short-chain organic acids to reduce the potential of postharvest decay. Plant Dis. 82: 689-693. 175. Sholberg, P.L. and Gaunce, A.P. 1995. Fumigation of fruit with acetic acid to prevent postharvest decay. Hortsci. 30: 1271-1275. 176. Sholberg, P.L. and Gaunce, A.P. 1996a. Fumigation of stone fruit with acetic acid to prevent postharvest decay. Crop Prot. 15: 681-686. 177. Sholberg, P.L. and Gaunce, A.P. 1996b. Fumigation of high moisture seed with acetic acid to control storage mold. Can. J. Plant Sci. 76: 551-555. 178. Sholberg, P.L., Reynolds, A.G., and Gaunce, A.P. 1996. Fumigation of table grapes with acetic acid to prevent postharvest decay. Plant Dis. 80: 1425-1428. 179. Sinha, R.P. 1986. Toxicity of organic acids for repair-deficient strains of Escherichia coli. Appl. Environ. Microbiol. 51: 1364-1366. 180. Siragusa, G.R. 1995. The effectiveness of carcass decontamination systems for controlling the presence of pathogens on the surfaces of meat animal carcasses. J. Food Safety 15: 229-238.
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I. INTRODUCTION Citric acid is used in industry for a variety of purposes. It plays an important role in the food and beverage industry, as well as in the manufacture of pharmaceuticals and cosmetics. The global production of citrate during 1990s was estimated at around 500 metric tons with an increasing demand. Citric acid was first isolated from lemon juice by Swedish chemist Scheele in 1784. The John and Edmund Sturge Company successfully introduced the early commercial production of citric acid. Although citric acid was produced initially from citrus fruits, due to increasing demand, alternative methods of production were explored. Grimoux and Adam (1880) synthesized citric acid from glycerol. Wehmer (1919) produced citric acid by a fungal fermentation process using Penicillium species. In 1917, Currie used Aspergillus niger to produce citric acid in a high yielding fermentation process. Currie transferred this technology to Pfizer Company to establish the first commercial fermentation process for citric acid. Many changes have taken place in the technology since its inception. Among various substrates, beet molasses was found economical for large-scale production. Doelger and Prescott (1939) used static medium containing sucrose and inorganic salts to grow Aspergillus. In 1949, Perlman reported development of submerged fermentation processes using Aspergillus and molasses. Since1965, different methods including yeast-based fermentation processes were developed. It is interesting to note that only a small amount of citric acid is produced from citrus fruits. Citrate is widely used as an acidulant in beverages, confectionery, and effervescent salts; in pharmaceutical syrups, elixirs, in effervescent powders and tablets, to adjust the pH of foods and as synergistic antioxidant, in processing cheese. Also used as an additive in beverages, jellies, jams, preserves and candy to provide tartness. For non-dietary applications, citrate is used in the manufacture of alkylated resins; in esterified form as plasticizer, and foam inhibitor. Citrate is also used for sequestering color; in electroplating; in special inks; in analytical chemistry for determining citrate-soluble P2O5; as a reagent for albumin, mucin, lactoferrin, glucose, and bile pigments. In hematology, citrate
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is widely used as a component of anticoagulant solutions (citrate dextrose solution; citrate phosphate dextrose solution; and citric acid syrup).
II. OCCURRENCE AND PROPERTIES A. Biosynthesis Citric acid is produced as a bio-active molecule by plants and animals during metabolism. Acetyl-CoA derived from the oxidation of carbohydrates, fatty acids and amino acids during catabolism enters the tricarboxylic acid cycle. In this cycle, at each turn one molecule of acetic acid enters as acetyl CoA and condenses with a molecule of 4-Carbon oxaloacetic acid to form the 6-Carbon tricarboxylic compound ‘citric acid’. Acetyl-CoA + Oxaloacetic acid Citroyl-CoA Citric acid + CoASH The rate of this reaction is largely determined by the availability of acetyl-CoA, oxaloacetate and the concentration of succinyl-CoA, which competes with acetyl-CoA and inhibits citrate synthase. Aspergillus, yeasts, and certain bacteria accumulate citric acid in large quantities. Although such accumulation does not occur in normal physiological processes, it is found among mutants or strains with altered metabolic pathways. The addition of specific nutrients as well as selection of substrates paves the way for such production (Clark, 1962; Clark et al., 1965). B. Fermentation It is generally accepted that a rapid flux of carbon through glycolysis to pyruvate and a restriction in tricarboxylic acid cycle prevents the breakdown of citric acid once it is formed and results in the rapid accumulation of citric acid. Netik et al. (1997) reported that the cellular uptake and export of citric acid by Aspergillus niger occurs by active, H(+)-symport dependent systems. These systems are inhibited by metabolizable tricarboxylic acid analogs and pthalic acid, and by several other mono- di-, and tri-basic organic acids. Citrate export is demonstrated in mycelia cultivated under manganese-deficient conditions, whereas the uptake of citrate from media was only detectable during pre-cultivation of A. niger in media supplemented with manganese ions. C. Properties Chemical nomenclature: 2-Hydroxy-1,2,3-propanetricarboxylic acid; β-hydroxytricarballylic acid. Chemical formula: C6H8O7; molecular weight: 192.13 (Carbon, 37.51%; Hydrogen, 4.20%; Oxygen, 58.29%). Citric acid is widely distributed in plants and in animal tissues and fluids. As a monohydrate, citrate forms ortho-rhombic crystals in cold aqueous solution. Citrate has a pleasant, sour taste. The monohydrate crystals lose water in dry air or when heated at about 40 to 50˚C, and are slightly deliquescent in moist air. It softens at 75˚C with melting point ≈100˚C. A 0.1N citrate solution has a pH of 2.2. Citric acid is a pure white crystalline solid. Citrate salts of ammonium, sodium and potassium are all highly soluble in water and are weak alkalines. The physico-chemical properties of citric acid are listed in TABLE 1.
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TABLE 1. Citric acid - Physico-chemical properties Molecular weight Amorphous form 192.1 Hydrated form 210.1 Melting point 153˚C Solubility 146 g dissolves in 1 L water at 20˚C 525 g at dissolves in 1 liter water at 100˚C 62 g dissolves in 1 liter ethanol at 25˚C 2.25 g at 15˚C in esters Dissociation constant pK1 3.14 pK2 4.77 pK3 6.40
D. Assays The methods of analysis according to the Association of Official Analytical Chemists (Williams, 1984) describes chemical assays for detection and quantitation of various acids in foods. Assays for organic acids in foods are generally carried out for three reasons: i) organic acid is a natural component of the product and therefore the assay is a quantitative or qualitative measure of wholesomeness or lack of adulteration or is a confirmation of the standard of identity for that product; ii) acid is not normally present in the food product or is present at levels lower than that normally detected in a standard assay and serves as a measure of adulteration either through addition of the acid or fermentation of the substrate to form acidic by-products; and iii) organic acid is added to achieve a desired effect as regulated by Good Manufacturing Practice (GMP). In general, methods in practice are dependent on ease of separation of citrate from the food, the food product itself, and the desire for quantitative or qualitative results. It is desirable to estimate the levels of acetic and propionic acids in breads and cakes, eggs, and seafood; citric acid in wines, cheese, and dried milk. In the case of organic acids, enzymatic analysis for acetic, citric, isocitric, L-and D-lactic, L-malic, and succinic acids can be performed to identify citric acid (Bergmeyer, 1974). Acids are also quantitated using paper chromatography (Tijan & Jansen, 1971), gas chromatography (Martin et al., 1971), and high performance liquid chromatography (HPLC) (Marsili et al., 1981).
III. ANTIMICROBIAL ACTIVITY Citric acid, like many other organic acids, elicits antimicrobial activity by various mechanisms. The antimicrobial outcome is influenced by various factors including pH, concentration, temperature, chain length etc. In addition to the antimicrobial property, the choice of the acidulant may depend upon secondary activity. Citric acid contributes to the taste and tartness of a product. It may create a synergistic relationship with antioxidants by chelating metal ions. It can control pectin gel formation, aid in the inversion of sucrose, prevent browning, and protect color. Certain citrate formulations find use as chemical leavening agents. Salts of acids may be important in regulating the acidity of foods. Although citric acid is not used solely for its antimicrobial activity, it is shown to exhibit certain antimicrobial properties against molds and bacteria. In 1950, Murdock reported that some of the organisms isolated from tomato juice were inhibited by citric
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acid. Fabian and Graham (1953) found that citric acid was the more inhibitory to thermophilic bacteria than acetic and lactic acids. Further studies showed that pH was not a reliable indicator to measure preservation efficacy (Fabian & Wadsworth, 1939). Canned tomatoes acidified with citric, fumaric and malic acids did not show significant differences in their physical or chemical quality (Schoenemann & Lopez, 1973; Schoenemann et al., 1974). Concentrations of 12-12.5% sodium citrate were inhibitory to Salmonella Anatum and Salmonella Oranienburg (Davis & Barnes, 1952). Thomson et al. (1967) found that 0.3% citric acid could reduce viable Salmonella on poultry carcasses. Skim milk acidified with citric acid was the most inhibitory to Salmonella Typhimurium followed by lactic and hydrochloric acids (Subramanian & Marth, 1968). Staphylococcus aureus is inhibited by increasing concentrations of citric acid and decreasing pH (Minor & Marth, 1970). Sodium citrate could elicit bacteriostatic activity. Sodium citrate in concentrations of 0.1-4.0% was not as inhibitory to Streptococcus agalactiae when added to skim milk or fresh milk as citric acid at concentrations of 1, 2, and 4. This phenomenon seems due to a reduced pH effect rather than chelation of magnesium ions in the milieu (Sinha et al., 1968). The antimicrobial activity of citrates has been attributed to its ability to chelate metal ions (Barnen & Keenan, 1970). Lactobacillus casei is inhibited by sodium citrate induced metal-chelation at 12-18 µM concentrations. Chelation effect also appears to be an influencing factor in the growth-inhibition of Staphylococcus aureus (Rammell, 1962) and Arthrobacter pascens (Imai et al., 1970). Ahamad and Marth (1990) examined the ability of acetic, citric and lactic acid to prevent growth of Listeria monocytogenes in TB during extended incubation at 7-35˚C. Citric aid was less inhibitory than acetic acid, with growth of listeriae occurring in all samples with 0.1% citric acid regardless of temperature. Based on average minimum pH values permitting growth of four L. monocytogenes strains at 10, 20, and 35˚C, Sorrells and others found that acetic acid was again most inhibitory (pH 5.04) followed by lactic (pH 4.73), citric (pH 4.53), malic (pH 4.46) and hydrochloric acids (pH 4.46). Citric and lactic acids have different effects on survival of listeriae. Although high levels of both acids inactivated listeriae in a similar pattern, low levels (0.1-0.5 M) of citric acid, especially at pH 5-6, protected listeriae from death (El-Gazzar & Marth, 1991; Buchanan et al., 1993; 1994). From the studies of Young and Foegeding (1993), it can be inferred that at the same pH levels, growth of listeria was affected most by acetic acid, followed by lactic and citric acids. The inhibitory effects of different salts of weak acids also were similar, with acetates being more inhibitory than lactates and citrates exhibiting the weakest action (Kouassi & Shelef, 1996). Post et al. (1985) observed no change in numbers of Clostridium botulinum in tomato puree, shrimp puree acidified with citric or acetic acids to pH 4.2 or 4.6. No toxins were detected in any of these foods for up to 8 weeks. Similarly Tsang et al. (1985) found neither growth nor toxin production in TPGY medium acidified to pH 100-fold increase in cell numbers) was the same at 30˚C but elevated to 4.83 at 10˚C and 7.0 at 5˚C. L. monocytogenes survived low pH values better at lower temperatures. These experiments used citrate phosphate buffer in which the citric acid content was calculated as 1.1% at pH 4.4 and 0.7% at pH 6.0. The authors suggested that the inhibitory activity might be due to the chelating ability of citric acid. Additional interactive effects were also observed in the presence of salt. Using the multiple-barrier concept, hard-cooked eggs allowed to equilibrate in 0.5, 0.75, or 1.0% concentrations of citric acid and 0.2% sodium benzoate were held for 30 days at 4˚C, or in 0.75% citric acid alone for 21 days at 4˚C. A concentration of 0.75% citric acid was sufficient to reduce inoculated populations of Salmonella Typhimurium, Yersinia enterocolitica, Escherichia coli, and S. aureus (Fischer et al., 1985). Daly et al. (1973) used a combination of 0.1% citric acid and 0.75% gluconolactone incorporated into sausage before fermentation. This combination inhibited the growth of S. aureus early in the fermentation, and the increased acidity of the meat mixture allowed the fermentation to proceed more quickly. Restaino et al. (1982) used a combination of 0.05% potassium sorbate and citric acid at pH 5.0 to reduce the growth rate of Saccharomyces rouxii and Saccharomyces bisporus. Potassium sorbate at 0.2% concentration in combination with citric and lactic acid at pH 5.5 suppressed the growth of Lactobacillus plantarum but did not effect Pseudomonas aeruginosa (Resatino et al., 1981). Citric acid is also known to limit growth production of Aspergillus parasiticus and A. versicolor. At a level of 0.75% both citric acid and lactic acids had a slight growth retarding effect on A. parasiticus. At 0.25% toxin production was greatly reduced. 0.5% citric acid inhibited the growth and at 0.25% toxin production was suppressed. Even a concentration of 0.75% of citric or lactic acids did not affect the growth of Penicillium expansum (Reiss, 1976) Beelman et al. (1989) developed an acid-blanch-chelate (ABC) process designed to reduce mesophilic and thermophilic bacterial spoilage in canned mushrooms. They demonstrated that acid blanching in a citric acid (0.05 M) solution buffered to pH 3.5 enhanced inhibitory activity during processing. This process also reduced thermophilic spoilage from 68 to 23.9% by adding citric acid to can brine, which was further reduced to 16.8% by the addition of EDTA. Some studies have demonstrated a synergism between citric acid, polyphosphoric and EDTA with antimicrobials such as monolaurin, monocarpin, sucrose dicaprylate and sucrose monolaurate, thus exhibiting a high antibacterial activity against E. coli and other Gram-negative bacteria. It was concluded that the transport of monolaurin into the cell membrane of E. coli was enhanced by the action of citric, polyphosphoric acids and EDTA (Shibsaki & Kato, 1978; Blaszyk & Holley, 1998). Nickerson and Darak (1978) described a composition and method for safely extending the storage life of refrigerated foods, such as shelled, hard-cooked eggs, cooked peeled shrimp, cooked and uncooked shrimp and cooked mushroom. The technique is based on applying mixtures of preservatives with a buffering agent such as citric and/or phosphoric acids. A buffering agent is needed in amounts to maintain the pH of the solution in the range of approximately 4.5 to 5.5 and selected from the group consisting of
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both citric acid and sodium or potassium hydroxide, or a mixture of sodium or potassium monohydrogen phosphate, dihydrogen phosphate or phosphoric acid. The fate of Salmonella Enteridis PT4 in home-made mayonnaise prepared with citric acid solution [citric acid concentration of ≥ 4.98% (w/v)] was investigated (Xiong et al., 1999). It was found that the pH of mayonnaise is closely related to the ratio of egg yolk to citric acid, and the inactivation rate of the microorganisms increased as the ratio decreased and/or incubation temperature increased. To achieve a Salmonella Enteritidis PT4-free home-made mayonnaise, it was recommended to prepare with pure lemon juice [citric acid concentration ≥ 5%(w/v)], and the pH should be 3.30 or below, or, in practice, at least 20 ml pure lemon juice per fresh egg yolk should be used. Silla-Santos et al. (1995; 1996) found that citric acid has a stronger inhibiting effect than glucano-delta-lactone on the recovery of Clostridium sporogenes PA 3679 spores. In an earlier experiment these authors compared glucono-delta-lactone and citric acid as acidulants for lowering the heat resistance of Clostridium sporogenes PA 3679 in HTST working conditions. Citric acid was more effective in reducing the heat resistance of spores than GDL at all of the temperatures. The reduction in pH diminished the value of the ‘z’ parameter, although it was necessary to lower the pH to 4.5 to obtain a significant reduction. El-Shenawy and Marth (1989; 1991; 1992) investigated the anti-listerial activity at 13 and 35˚C of sodium propionate in combination with common organic acids. TB was prepared to contain 0, 500, 1500, or 3000 ppm sodium propionate and the pH of the medium was adjusted to 5.0 or 5.6 with HCl, or one of four common organic acids (acetic, tartaric, lactic, and citric). Decreasing the pH from 5.6 to 5.0 enhanced the anti-listerial activity of propionate. Organic acids, when compared with HCl, greatly enhanced the anti-listerial activity of propionate, with acetic acid being the most effective followed by tartaric, lactic and citric acids. In a subsequent study, the same authors investigated the antibacterial activity of sorbate in the presence of other organic acids. TB was prepared to contain 500, 1500, and 3000 ppm potassium sorbate and pH of the medium was adjusted to 5.0 or 5.6 using HCI or organic acids (acetic, tartaric, lactic or citric), inoculated with L. monocytogenes, and incubated at 13 or 35˚C. When compared with HCl as an acidulant, the anti-listerial activity of sorbate was enhanced more by organic acids, with acetic and tartaric acids being more effective than lactic and citric acids. Sheldon and Schuman (1996) reported that when stored at 4˚C, L. monocytogenes populations in an inoculated commercially available reduced-cholesterol liquid whole egg product could be reduced as much as 3.9 orders of magnitude by adjusting the pH of the product to 6.6 with citric acid and adding nisin at a level of 1000 IU/mL. Yamaguchi et al. (1996) investigated various properties of citric acid and EDTA solution as decalcifying and cleansing agents in root canal irrigation, as well their antibacterial effects. Citric acid solution was found to exhibit antibacterial effects on the bacteria used.
IV. APPLICATIONS A. Clinical applications A unique application of citric acid was studied by Marazova et al (1997). They studied the effect of newly synthesized agent MX1, a salt of active metabolite of the H2blocker roxatidine with a complex of bismuth and citric acid against restraint ulcers. The experiments, conducted on rats, showed that MX1 has a gastroprotective effect, but also
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showed that bismuth subcitrate significantly reduced the ulcer size when higher doses are employed (Marzova et al, 1997). Topical citric acid produces notable changes very similar to those produced in response to glycolic acid, ammonium lactate, and retinoic acid including increases in epidermal and dermal glycosaminoglycans and viable epidermal thickness (Bernstein et al, 1997). Renvert et al. (1997) evaluated subgingival irrigation with citric acid using an enzyme immunoassay. Subgingival irrigation is sought to be a supplement to scaling and root planing. Citric acid irrigation had no assurable microbiological effects. In another study Domiguez (1997) demonstrated that citric acid solution, used as a test drink, is superior to the previously proposed semi-liquid test meals in terms of the production of 13CO -urea breath for the diagnosis of Helicobacter pylori infection. 2 Nagoba et al. (1998) recently studied a possible treatment of superficial pseudomonal infections with citric acid. The authors feel that the treatment was both effective and cheaper than the conventional methods. Most current dentin bonding procedures use acid etchants to partially demineralize the dentin structure and provide pathways for resin infiltration. On rehydration, the dehydrated surfaces underwent an expansion up to level seen after etching and tubule diameters returned to the etched values. These results indicate that the collapse of demineralized matrix is almost totally recoverable on rehydration (Marshall et al, 1998). B. Dietary applications The effect of dietary citric acid supplementation on calcium and phosphorus bioavailability in rats showed that citric acid increased intestinal absorption of calcium and phosphorus (Lacour et al., 1997). The study also showed that prolonged administration of calcium citrate supplements may help increase bone mineral concentration. C. Pharmaceutical applications In pharmaceutical industry citric acid is included in the formulation for many types of effervescent tablets, producing effervescent effects when it reacts with carbonates or bicarbonates. Citric acid is also used for its weak acidic nature, when the active agent is a basic substance. Trisodium citrate is used routinely as a blood anticoagulant. It complexes with calcium, one of the requirement to complete clotting. In cosmetics industry, citric acid is added in several creams, ointments, and shampoos. Zinc citrate is used in toothpastes for its antibacterial and antiplaque properties.
V. INDUSTRIAL PRODUCTION A. Production processes Currently, there are two organisms that are widely used in the production of citric acid, i.e. yeast and Aspergillus niger. Many other fungi are also able to produce citric acid such as A. clavatus, A fumigatus, A. citrinum and Candida species. Yeast has certain advantages over Aspergillus due to its independence with trace metals and higher fermentation rates. It also has the potential for higher sugar concentrations using osmophilic variants (Pfizer Inc. 1974). Citric acid is produced by a number of different processes mainly by submerged liquid fermentation, liquid-surface and koji methods (Kubicek & Rohr, 1986; Kristiansen & Sinclair, 1979).
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1. Submerged liquid fermentation process. Submerged liquid fermentation is one of the important and probably the most popular method used for the production of citric acid (Hustede & Rudy, 1976a; 1976b). A suitable substrate such as beet molasses, glucose syrup is sterilized and inoculated with a strain of Aspergillus. The inoculum can be introduced directly as spores or in vegetative form. The vital part lies in the actual morphology of the hyphae and the subsequent aggregation to form small spherical pellets. The hyphae should be abnormally short arising out of the deficiency of the manganese (Kisser et al., 1980). Factors resulting in the production of such pellets are the correct ferrocyanide level (Clark, 1964) and the correct concentration of manganese (Clark, 1966). The medium is aerated or aerated and agitated depending on the type of fermenter tank used. A period of growth phase, during which almost no citric acid is produced, is followed by a production phase. In this phase the cells do not grow any longer and the entire substrate is now made available for citric acid production. The fermentation time is usually 2 - 5 days. Temperature and pH are accurately controlled. Initial pH is usually between 5 and 7, although final pH is around 2.0. Oxygen content is maintained at 10%, air saturation at 12%. 2. Liquid surface process. This process was first developed by Pfizer (1974). In this method, the fermentation is carried out in shallow trays with suitable medium. Beet molasses are used as a source for carbohydrates. pH is regulated to around 5.0, and additional nutrients are added, before the medium is sterilized. It is then inoculated with Aspergillus and left at a temperature of 30˚C. The room is kept aerated so that oxygen supply is unhindered. Since the absorption of oxygen in to the cells is by surface aeration only, the whole process is completed in 7-12 days. At the end of the process, the mycelial mat formed is separated from the liquid. This liquid contains citric acid which is then purified. 3. Koji process. This process is almost exclusively employed in Japan. The main features are the use of sterilized wheat bran or sweet potato waste, giving a final water concentration of 70 - 80%, which is then inoculated with spores of A. niger and spread out in trays. The place is aerated and temperature maintained at around 28˚C. The entire process is finished in a week, and after the mash is removed citric acid is extracted. The effect of pH value, methanol, and salt concentration on the production of citric acid from cheese whey by two strains of Aspergillus niger (CAIM 111 and CAIM 167) was investigated by Samragy et al. (1996). The cumulative effect of fermentation medium pH (3.5), methanol concentration (4% v/v) and salt concentration (10%, w/v) during the fermentation process of whey did not enhance the production of citric acid by A. niger CAIM 111, while it did increase the production of citric acid by A. niger CAIM 167 by 4 times. Influence of calcium on fungal growth, hyphal morphology and citric acid production in Aspergillus niger was studied by Pera and Callieri (1997). Addition of 0.5g/L CaCl2 to the fermentation medium lowered the final biomass dry mass by 35% and increased the uptake of phosphate and sucrose, and the production of citric acid by 15, 35 and 50% respectively. Changes in the process which alter the Aspergillus niger metabolism during citric acid fermentation was studied by Legisa et al. (1995), by altering the substrate and by application of different substances at different concentrations. Initially, a higher sucrose
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concentration was used for the germination of spores, which caused a higher intracellular level of the osmo-regulator, glycerol, to be present. When citric acid started to be excreted into the medium, the substrate was suddenly diluted. This, the authors reasoned, induced the increased citric acid production. Kirimura et al. (1999) described a method for the production of citric acid from xylan hydrolysate cultivated in a semi-solid culture of Aspergillus niger. They were able to directly produce 39.6 g/L of citric acid maximally in 3 d from 140 g/L of xylan. B. Product recovery After the organism synthesizes and accumulates citric acid and it is removed from the final broth, the product can be recovered by one of the two methods that are generally applied—The classical recovery method or the solvent extraction method (Marison, 1988; Sirman et al., 1990). 1. Classical recovery method. When molasses-based fermentation is used for manufacture of citric acid, impurities originate from the substrate. So, it is essential to purify and recover citric acid. The fermented broth is heated and lime is added. This precipitates insoluble calcium citrate trihydrate, which is then washed and treated with sulfuric acid. It releases citric acid and the calcium sulfate is removed. 2. Solvent extraction method. This method is employed when cleaner feedstocks are used in manufacturing process. This process involves removal of citric acid from the broth by treating it with the solvent at a low temperature followed by subsequent removal of the acids at a high temperature. Extractants used include butan-2-ol and tributyl phosphate diluted with small quantity of kerosene.
VI. SAFETY AND TOLERANCE Toxicological data in animal models show different tolerance levels depending on the route of administration. Yokotani et al. (1971) tested the toxicity of commercial citric acid. The LD50 for mice administered by oral route is 5.0-5.8 g, subcutaneous is 2.7 g and for intravenous is around 0.95 g per kg body weight. For rat toxicity through oral administration the LD50 is 11.7 g and subcutaneous is 5.5 g per kg body weight. Death resulted due to respiratory or cardiac failure and hemorrhage of gastric mucosa. Gruber and Halbeisen (1948) inferred that the symptoms were similar to that of calcium deficiency. Studies conducted by Horn et al. (1957) showed that death of mice resulted from acute acidosis and hemorrhages of respiratory organs when citrate was administered by intravenous route. Short-term studies on rats fed 0.2, 2.4, and 4.8% citric acid in a commercial diet showed lowered weight gains as a result of decreased intake of food, and slight blood chemistry abnormalities at the 4.8% level; slight atrophy occurred in regions of the thymus and spleen (Yokotani et al., 1971). Long-term feeding studies with rats fed quantities up to 5% citric acid showed no significant changes from control groups (Bonting & Jansen, 1956; Horn et al., 1957). Cramer and co-workers (1956) investigated the relationship of the intake of sodium citrate and citric acid in vitamin D free diets containing low levels of phosphorus but ade-
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quate levels of calcium. When vitamin D was not given, the citrate completely prevented the absorption of calcium. Although there was no effect on weight gain, the urine contained calcium citrate. The authors concluded that citrate had a rachitogenic effect on the test animals. Gomari and Gulyas (1944) administered 0.32-1.20 g/kg body weight of sodium citrate to dogs, which left the blood calcium levels unchanged but at the same time increased the urine calcium. Gruber and Halbeisen (1948) concluded that when citrate salts were administrated the acid part of the molecule was responsible for toxicity rather than the citrate moiety.
VII. REGULATORY STATUS Citric acid is universally accepted as a safe food ingredient. With a pleasant sour taste, it has found its way into several foods and beverages. It is highly soluble in water and enhances the flavor of citrus-based foods. The Food and Drug Administration lists citric acid and its sodium, potassium and calcium salts, as multipurpose Generally Recognized As Safe (GRAS) food additives. The joint FAO/WHO (JEFCA) has allocated to citric acid an Acceptable Daily Intake (ADI) of ‘Non-specified’ category. This means that, on the basis of the available data (chemical, biochemical, toxicological and others), the total daily intake of the substance, arising from its use at the levels required to achieve the desired effect, does not represent a hazard to health. Citric is also used in countering oxidative discoloration of meats and fruits and other foods. When used in accordance with good manufacturing practice, citric acid may be used as a sequestrant. (21 CFR§182.6033). The calcium, sodium and potassium salts of citric acid, and isopropyl citrate at less than 0.02%, monoisopropyl citrate and stearyl citrate are commonly used as sequestrants. Monoglyceride citrate is used in antioxidant formulations for addition to oils and fats at less than ppm of the combined weight of the additive and fat or oil. Triethyl citrate is used in dried egg whites at levels less than 0.25%. An iron-choline-citrate complex may be used as a source of iron in foods for special dietary use. Iron ammonium citrate is used as an anti-caking agent in salt for human consumption when the level of the additive does not exceed 25 ppm in the finished product. Citric acid is also used as an acidulant in carbonated beverages for citrus flavor. Sodium citrate and tartrate are used as chelating agents to prepare noncaking, meat-salt mixtures (Gardner, 1966; 1972).
VIII. SUMMARY Most plants and animals produce citric acid during metabolism. The tartness of the citrus fruits is due to the citric acid. Lemon juice contains 4 - 8% and orange has about 1% citric acid. Citric acid is widely used in foods, pharmaceuticals, and cosmetics. Citric acid has gained universal acceptance as a GRAS ingredient and the Joint FAO/WHO committee (JEFCA) has not set any ADI value. Although not a direct antimicrobial agent, citrate is recognized for enhancing the antimicrobial property of many other substances, either by reducing pH or by chelation of metal ions. Its use in controlling thermophiles, in particular, is well established. Citric acid is also used as an antioxidant to prevent oxida-
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tive discoloration in foods such as meats, fruits, and potatoes. Citrates of sodium, potassium and calcium also are recognized as GRAS ingredients with a wide range of food applications.
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Ahamad, N., and Marth, E.H. 1987. Behavior of Listeria monocytogenes at 7, 13, 21, and 35°C in tryptic soy broth acidified with acetic, citric or lactic acid. J. Food Prot. 52:688-695. Beelman, R.B., Witowski, M. E., Doores, S. Kilara, A., and Kuhn, G. D. 1989. Acidification process technology to control thermophilic spoilage in canned mushrooms. J. Food Prot. 52:178. Bergmeyer, H.U.1974. Methods of Enzymatic Analysis, vols.1 and 2. New York: Academic Press. Bernstein, E.F., Underhill, C.B., Lakkakorpi, J., Ditre, C.M., Uitto, J., Yu, R.J., and Scott, E.V. 1997. Citric acid increases viable epidermal thickness and glycosaminoglycan content of sun-damaged skin. Dermatol. Surg. 23:689-694. Blaszyk, M., and Holley, R.A. 1998. Interaction of monolaurin, eugenol and sodium citrate on growth of common meat spoilage and pathogenic organisms. Int. J. Food Microbiol. 39:175-183. Bonting, S.L., and Jansen, B. C. P. 1956. The effect of a prolonged intake of phosphoric acid and citric acid in rats. Voeding 17:137. Branen, A.L., and Keenan, T.W. 1970. Growth stimulation of Lactobacillus casei by sodium citrate. J. Dairy Sci. 53:593-597. Buchanan, R.L., and Golden, M.H. 1994. Interaction of citric acid concentration and pH on the kinetics of Listeria monocytogenes inactivation. J. Food Prot. 57:567-570. Buchanan, R.L., Golden, M.H., and Whiting, R.C. 1993. Differentiation of the effects of pH and lactic or acetic acid concentration on the kinetics of Listeria monocytogenes inactivation. J. Food Prot. 56:474-478. Clark, D.S. 1962. Submerged citric acid fermentation of ferrocyanide treated beet molasses: Morphology of pellets of A. niger. Can J. Microbiol. 8:133-136. Clark, D.S. 1964. Citric acid production, United States Patent No.3,118,821. Chem. Abstr. 61 4926d. Clark, D.S., Ito, K., and Horitsu, H. 1966. Effect of manganese and other heavy metals on submerged citric acid fermentation of molasses. Biotechnol. Bioeng. 8:465-471. Clark, D.S., Ito, K., and Tymchuck, P. 1965. Effect of potassium ferrocyanide addition on the chemical composition of molasses mash used in the citric acid fermentation. Biotechnol. Bioeng. 7:269-278. Cole, M.B., Jones, M.V., and Holyoak C. 1990. The effect of pH, salt concentration and temperature on the survival and growth of Listeria monocytogenes. J. Appl. Bacteriol. 69:63. Cramer, J.W., Porrata-Doria, E. I., and Steenbock, H. 1956. A rachitogenic and growth-promoting effect of citrate. Arch. Biochem. Biophys. 60:58-63. Currie, J.N. 1917. The citric acid fermentation of A.niger. J. Biol. Chem. 31:15-17. Daly, C., Lachance, M., Sandine, W. E., and Elliker, P. R. 1973. Control of Staphylococcus aureus in sausage by starter cultures and chemical acidulation. J. Food Sci. 38:426. Davis, F., and Barnes, L.A. 1952. Suppression of growth of Salmonella anatum and Salmonella oranienburg by concentration variation of energy sources in a synthetic basal medium. J. Bacteriol. 63:33-38. Dominguez, M. J. E., Leodolter, A., Sauerbruch, T., and Malfertheiner, P. 1997. A citric acid solution is an optimal drink in the 13C-urea breath test for the diagnosis of Helicobacter pylori. Gut 40:459-62. Doulger, W.P., and Prescot, S.C. 1939. Citric acid fermentation. Ind. Eng. Chem. 26:1142-1149. El-Gazzar, F.E., and Marth, E.H. 1991. Survival of Listeria monocytogenes in food colorant derived from red beets. J. Dairy Sci. 74:81-85. El-Shenawy, M.A., and Marth, E.H. 1989. Inhibition and inactivation of Listeria monocytogenes by sodium benzoate together with some organic acids. J. Food Prot. 52:771-776. El-Shenawy, M.A., and Marth, E.H. 1991. Organic acids enhance the antilisterial activity of potassium sorbate. J. Food Prot. 54:593-597. El-Shenawy, M.A., and Marth, E.H. 1992. Behavior of Listeria monoytogenes in the presence of sodium propionate together with food acids. J. Food Prot. 55:241-245. Fabian, F. W., and Graham, H. T. 1953. Viability of thermophilic bacteria in the presence of varying concentrations of acids, sodium chloride and sugars. Food Technol. 7:212-217. Fabian, F. W., and Wadsworth, C. K. 1939b. Experimental work on lactic acid in preserving pickles and pickle products. II. Preserving value of acetic acid and lactic acid in the presence of sucrose. Food Res. 4: 511-519.
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27.
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FAO/WHO. 1963. Specifications for the Identity and Purity of Food Additives and Their Toxicological Evaluation: Emulsifiers, Stabilizers, Bleaching and Maturing agents. 7th Report of the Joint Food and Agriculture Organization of the United Nations/World Health Organization Expert Committee on Food Additives. WHO Tech. Report Ser. No. 281. FAO Nutrition Meetings Report Ser No.35. FAO/WHO. 1973. Toxicological Evaluation of Certain Food Additives with a Review of General Principles and of Specifications. 17th Report of the Joint Food and Agriculture Organization of the United Nations/World Health Organization Expert Committee on Food Additives. WHO Tech. Report Ser. No.539. FAO Nutrition Meetings Report Ser. No. 53. Fischer, J. R., Fletcher, D.L., Cox, N. A., and Bailey, J.S. 1985. Microbiological properties of hard-cooked eggs in a citric acid-based preservation solution. J. Food Prot. 48:252. Gardner, W. H. 1972. Acidulants in food processing. In Handbook of Food Additives, 2nd ed., ed. T.E. Furia, pp.225. Cleveland, OH: CRC Press. Gardner, W.H. 1966. Food Acidulants. New York: Allied Chemical Corporation. Gomori, G., and Gulyas, E. 1944. Effect of parenterally administered citrate on the renal excretion of calcium. Proc. Soc. Exp. Biol. Med. 56:226-228. Grimoux, E., and Adam, P. 1880. Synthase de l’acide citrique. C.R. Hebd Séance Acad. Sci. 90:1252-1255. Gruber, C.M., and Halbeisen W. A. 1948. A Study on the comparative toxic effects of citric acid and its sodium salts. J. Pharmacol. Exp. Ther. 94:65-67. Horn, H.J., Holland, E.G., and Hazelton, L. W. 1957. Safety of adipic acid as compared with citric and tartaric acid. J. Agr. Food Chem. 5:759-761. Hustede, H., and Rudy, H. 1976a. Manufacture of citric acid by submerged fermentation. United States Patent No. 3,941,656. Hustede, H., and Rudy, H. 1976b. Manufacture of citric acid by submerged fermentation. United States Patent No. 3,940,315. Imai, K., Banno, I., and Ujima, T. 1970. Inhibition of bacterial growth by citrate. J. Gen. Appl. Microbiol. 16:479-487. Kirimura, K., Watanabe, K., Sunagawa, T., and Usami, S. 1999. Citric acid production from xylan and xylan hydrolysate by semi-solid culture of Aspergillus niger. Biosci. Biotechnol. Biochem. 63:226-8. Kisser, M., Kubicek, C.P and Rohr, M. 1980. Influence of manganese on morphology and cell wall composition of A.niger during citric acid fermentation. Arch. Microbiol. 128:26-33. Kouassi, Y., and Shelef, L.A. 1996. Metabolic activities of Listeria monocytogenes in the presence of sodium propionate, acetate, lactate and citrate. 81:147-153. Kristiansen, B., and Sinclair, C.G. 1979. Production of citric acid in continuous culture. Biotechnol. Bioeng. 21:297-315. Kubicek, C.P., and Rohr, M. 1986. Citric acid fermentation. Crit. Rev. Biotechnol. 3:331. Lacour, B., Tardivel, S., and Druke, T. 1997. Stimulation by citric acid of calcium and phosphorous bioavailability in rats fed a calcium-rich diet. Miner. Electrolyte Metab. 23:79-87. Legisa, M., Gradisnik, G., and Grapulin, M. 1995. Sudden substrate dilution induces a higher rate of citric acid production by Aspergillus niger. Appl. Environ. Microbiol. 61:2732-2737. Marazova, K., Kloucheck, E., Popov, A., Ivanov, C.H., and Krushkov, I. 1997. Gastroprotective effect of MX1 (a novel salt of the active metabolite of roxatidine with a complex of bismuth and citric acid) against stress ulcers in rats. J. Pharm. Pharmacol. 49: 791-795. Marison, I.W. 1988. Citric acid production. In: Biotechnology for Engnieers: Biological Systems in Technological Processes, ed. A.H. Scragg, pp. 323-326. Chichester, England: Ellis Horwood. Marshall, G.W. Jr., Wu, Maigidi, I. C., Watanabe, L. G., Inai, N., Balooch, M., Kinney, J.H., and Marshall, S.J. 1998. Effect of citric acid concentration on dentin demineralization, dehydration, and rehydration: atomic force microscopy study. J. Biomed. Mater. Res. 42:500-507. Marsili, R.T., Ostapenko, H., Simons, R.E., and Green, D. E. 1981. High performance liquid chromatography determination of organic acids in dairy products. J. Food Sci. 46:52-57. Martin, S.M., and Waters, W.R. 1952. Production of citric acid by submerged fermentation. Ind. Eng. Chem. 44:2229-2240. Minor, T.E., and Marth, E. H. 1970. Growth of Staphylococcus aureus in acidified pasteurized milk. J. Milk Food Technol. 33:516. Murdock, D. I. 1950. Inhibitory action of citric acid on tomato juice flat sour organisms. Food Res. 15:107. Nagoba, B. S., Deshmukh, S. R., Wadher, B. J., Mahabaleshwar, L., Gandhi, R.C., Kulkarni, P.B., Mane, V.A., and Deshmukh, J. S. 1998. Treatment of superficial pseudomonal infections with citric acid. J. Hosp. Infect. 40:155-157.
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Netik, A., Torres, N.V., Riol, J.M., and Kubieck, C.P. 1997. Uptake and export of citric acid by Aspergillus niger is reciprocally regulated by manganese ions. Biochim. Biophys. Acta 1326:287-294. Nickerson, J.T.R., and Darack, J.R. 1978. US Patent 4076850. Notermans, S., Dufrenne, J., and Keybets, M.J.H. 1985. Use of preservatives to delay toxin formation by Clostridium botulinum (type B strain okra) in vacuum - packed, cooked potatoes. J. Food Prot. 48:851. Pera, L.M., and Callieri, D.A.1997. Influence of calcium on fungal growth, hyphal morphology and citric acid production in Aspergillus niger. Folia-Microbiol. 42:551-556. Perlman, D. 1949. Mycological production of citric acid - the submerged culture method. Econ. Bot. 3:360374. Pfizer Inc. 1974 Fermentation process for the production of citric acid. Br. Pat. 1,364,094. Chem. Abstr. 78: 70192y. Post, L. S., Amoroso, T.L., and Solberg, M. 1985. Inhibition of Clostridium botulinum type E in acidified food systems. J. Food Sci. 50:966. Rammell, C. G. 1962. Inhibition by citrate of the growth of coagulase positive staphylococci. J. Bacteriol. 84:1123. Reiss, J. 1976. Prevention of the formation of mycotoxins in whole wheat bread by citric acid and lactic acid. Experimentia 32:168. Renvert, S., Dahlen, G., and Snyder, B. 1997. Clinical and microbiological effects of subgingival antimicrobial irrigation with citric acid as evaluated by an enzyme immunoassay and culture analysis. J. Periodontol. 68:346-352. Restaino, L., Lenovich, L.M., and Bills, S. 1982. Effects of acids on potassium sorbate inhibition of foodrelated microorganisms in culture media. J. Food Sci. 47:134. Restaino., L., Komatsu, K.K., and Syracuse, M.J. 1981. Effects of acids and sorbate combinations on the growth of four osmophilic yeasts. J. Food Prot. 45:1138. Rohr, M., Zenhentgruber, O., and Kubicek, C.P., 1981, Kinetics of citric acid production by A.niger pilot plant scale. Biotechnol. Bioeng. 23:2433-2455. Samragy, Y. A., Khorshid, M. A., Foda, M.I., and Shehata, A.E., 1996. Effect of fermentation conditions on the production of citric acid from cheese whey by Aspergillus niger. Int. J. Food Microbiol. 29: 411416. Schoenemann, D.R., Lopez, A., and Cooler, F. W. 1974. pH and acidic stability during storage of acidified and nonacidified canned tomatoes. J. Food Sci. 39:257. Schoenemannn, D.R., and Lopez, A. 1973. Heat processing effects on physical and chemical characteristics of acidified canned tomatoes. J. Food Sci. 38:195. Sheldon, B.W., and Schuman, J.D. 1996. Thermal and biological treatments to control psychrotrophic pathogens. Poultry Sci. 75:1126-1132. Shibasaki, I., and Kato, N. 1978. In: The Pharmacological Effect of Lipids, ed. J.J. Kabara, pp.15. Champaign, IL: The American Oil Chemists Society. Silla, Santos, M.H., and Torres, Z. J. 1995. Glucono-delta-lactone and citric acid as acidulants for lowering the heat resistance of Clostridium sporogenes PA3679 in HTST working conditions. Int. J. Food Microbiol. 25:191-7. Silla, Santos, M.H., and Torres, Z. J. 1996. Evaluation of citric acid and GDL in the recovery at different pH levels of Clostridium sporogenes PA3679 spores subjected to HTST treatment conditions. Int. J. Food Microbiol. 29:241-54. Sinha, D.P., Drury, A.R., and Conner, G. H. 1968. The in vitro effect of citric acid and sodium citrate acid and sodium citrate on Streptococcus agalactiae in milk. Indian Vet. J. 45:805-810. Sirman, T., Pyle, D.L., and Grandison, A.S. 1990. Extraction of citric acid using a supported liquid membrane. In Separations for Biotechnology, ed. D. L. Pyle, pp. 245-254. London: Elsevier. Subramanian, C.S., and Marth, E. H. 1968. Multiplication of Salmonella typhimurium in skim milk with and without added hydrochloric, lactic and citric acids. J. Milk Food Technol. 31:323-326. Thomson, J.E., Banwart, G.J., Sanders, D.H., and Mercuri, A. J. 1967. Effect of chlorine, antibodies, propiolactone, acids and washing on Salmonella typhimurium on eviscerated fryer chickens. Poul. Sci. 46:146-151. Tijan, G.H., and Jamen, J.T.A. 1971. Identification of acetic, propionic, and sorbic acids in bakery products by thin layer chromatography. J. Assoc. Off. Anal. Chemists. 54:1150-1151. Tsang, N., Post, L. S. and Solberg, M. 1985. Growth and toxin production by Clostridium botulinum in model acidified systems. J. Food Sci. 50:961. Wehmer, C. 1919. Verlust des oxalsaure-bildungs-vermogens bei einem degenerierten Aspergillus niger. Zentrabl. Bacteriol. 49:145-148.
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Williams, S. 1984. Official Methods Analysis of the Association of Official Analytical Chemists, 14th ed. A.O.A.C., Arlington, Va. Xiong, R., Xie, G., and Edmondson, A. S. 1999. The fate of Salmonella enteritidis PT4 in homemade mayonnaise prepared with citric acid. Lett. Appl. Microbiol. 28:36-40. Yamaguchi, M., Yoshida, K., Suzuki, R., and Nakamura, H. 1996. Root canal irrigation with citric acid solution. J. Endodontics. 22:27-9. Yokotani, H., Usui, T., Nakaguchi, T., Kanabayashi, T., Tanda, M., and Aramaki, Y. 1971. Acute and subacute toxicological studies of TAKEDA-citric acid in mice and rats. J. Takeda Res. Lab. 30:25-35. Young, K.M., and P.M. Foegeding. 1993. Acetic, lactic and citric acids and pH inhibition of Listeria monocytogenes Scott A and the effect on intracellular pH. J. Appl. Bacteriol. 74: 515-520.
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Section-VI MILIEU-ANTIMICROBIALS
Sodium chloride Polyphosphates Chloro-cides Ozone
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I. INTRODUCTION Sodium chloride, commonly called salt, table salt, or rock salt, is a vital part of human life. The food that we eat is tasteless without salt. An average American consumes approximately 8-10 g of salt per day (Dickinson, 1980). Salt enhances the flavor of foods and plays a functional role in food processing. For instance, salt controls microbial growth and shifts the fermentation in a desirable direction in products like pickles and sauerkraut; it controls yeast activity, strengthens the gluten and enhances crust color in baking goods; it controls the lactic acid fermentation rate as well as enhances flavor, texture, ripening and shelf life extension in cheese; it lowers water activity, strengthens gel structure and enhances color in processed meats (Lynch, 1987). Apart from its use in the food industry, salt aids in road transportation during severe winter weather, where it is still the best method of ice removal. Salt is also widely used in the chemical industry. The history of salt dates back to the beginning of civilization, about 2700 BC, when one of the earliest known treatises on pharmacology, published in Chinese, contained information on several types of salt (Salt Institute, 1999). It has been referred to as the essence of life in Biblical teachings (Dickinson, 1980). Salt has been of economical importance in ancient history. In ancient Greece, goods were exchanged for salt. Salt tax has been an important issue of human history in many parts of the world. In Chinese history the salt tax was a major source of revenue (Salt Institute, 1999). Salt was a cause of the French Revolution. The salt tax supported British monarchs and people were imprisoned for smuggling salt. During the British rule in India, Mahatma Gandhi opposed the salt tax during the struggle for freedom. The desire for salt is believed to be an evolutionary process (Forsyth & Miller, 1980). It has been suggested that the neural-endocrine interactions in higher mammals play a role in behavior towards salt emergence and salinity control, and this relates to their parallel evolution (Denton, 1982). Studies on kangaroos living on the snowy mountains of Australia show a specific sodium appetite organized in the animals’ brains (Denton, 1982).
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Other related compounds of sodium that are used in food processing and preservation include sodium ascorbate, sodium benzoate, sodium bicarbonate, sodium citrate, sodium nitrate, sodium nitrite, sodium phosphate and sodium propionate. Some other salts that have been tried as a substitute for sodium chloride include potassium chloride, calcium chloride, ammonium chloride, magnesium chloride and lithium chloride. Each of these has limitations. Potassium chloride is the most closely related compound to sodium chloride, especially with regard to its physical and functional properties, but the limiting factor is its extreme bitter taste. Calcium and magnesium chlorides are very bitter too. Ammonium chloride is a highly unstable compound and lithium chloride is toxic to humans. Replacing sodium chloride partially with a mixture of potassium, magnesium and calcium chlorides in dry fermented sausage caused a decrease in saltiness (decrease in sensory acceptability) as well as an increase in acidity and water activity (Gimeno et al, 1998). The lactic acid bacteria were not affected, but the counts of Micrococcaceae decreased. However, partial replacement of sodium chloride with potassium lactate in dry fermented sausages did not cause significant sensory defects (Gou et al., 1996; Askar et al., 1993). Partial replacement of sodium chloride with magnesium chloride at low levels did not produce any sensorial defects in bologna (Seman et al., 1980) while in frankfurters magnesium chloride was not a suitable substitute (Hand et al., 1982). Substituting sodium chloride with glycine (above 40%) produced an unacceptable sweet taste and non-uniform texture (Gou et al., 1996). Potassium chloride has been used as a substitute in some formulations (Ibanez et al., 1995; 1996; 1997) while substitution of the same has caused significant bitterness in some others (Leak et al., 1987; Keeton, 1984). A 1:1 mixture of sodium and potassium chloride when fed to human subjects showed a reduction of sodium intake by 44-55% (Mickelson et al., 1972). Several seasonings and flavoring blends are also being tried as substitutes for sodium chloride. One such substitute included a mixture of potassium chloride, hydrolyzed vegetable protein, dipotassium orthophosphate, glucose, 5’-inosinic acid and 5’-guanosinic acid (Mohlenkamp & Miller, 1981). This blend was free of the bitter taste associated with potassium chloride. Autolyzed yeast blended with potassium chloride reduced the bitter taste due to potassium chloride (Shackelford, 1981). Another low sodium seasoning blend consisted of potassium chloride, monopotassium glutamate, potassium citrate, potassium phosphate, L-glutamic acid and silicon dioxide (Allen & Day, 1980). Glycinamide hydrochloride formed a good blend with monosodium glutamate (Sternberg et al., 1980). Addition of certain amino acids and their esters with sodium chloride has been found to enhance saltiness. L- ornithyl-B-alanine and Glycine ethyl ester hydrochloride enhanced the salty effect of sodium chloride (Okai et al., 1989). Some of the salty peptides included glycine methyl, ethyl ester hydrochlorides (Kawasaki et al., 1988) and L-ornithyltaurine (Tada et al., 1984).
II. OCCURRENCE AND PROPERTIES Salt is abundantly available in nature and has been designated as the fifth element, next to air, water, fire and earth (Dickinson, 1980). In the United States, salt deposits are found in the states of Michigan, Ohio, New York, Pennsylvania, Louisiana and Texas. The country has an annual production of about 22 millions of dry salt (Dickinson, 1980). Historically, salt was made by boiling brine from salt springs. In 1800,
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large-scale production of salt began and the first underground salt mine was found in 1869 (Salt Institute, 1999). Salt is produced by three methods (Dickinson, 1980). Recovering the rock salt by digging 600 to 2000 feet below the surface of the earth is called mining. Explosives are used to loosen the salt embedded in the rocks in the mines. Another method is removing the brine from brine wells using pipes, wherein, a pipe flushes water into a salt deposit and the brine formed is removed and brought to the surface using another pipe. The water is then evaporated or removed by heat, which leaves salt granules or flakes. The third method is natural evaporation of water from concentrated brines by sunshine, producing solar salt. The brine is concentrated in ponds to a point where it crystallizes and evaporates to form a salt bed. The crystallized salt is then harvested, washed and screened. This method can be only used in areas of heavy sunshine, very little rain and good air motion. In the United States, the sources of solar salt include the great Salt Lake in Utah, as well as the San Francisco Bay and San Diego areas in California. Salt as a chemical compound is made of two elemental substances, the cationic sodium ion (Na+) and the anionic chloride ion (Cl-), which react together forming the halide salt, sodium chloride. The role of sodium ion in the human body is to maintain the blood volume and cellular osmotic pressure as well as aiding in the transmission of nerve impulses (Institute of Food Technologists, 1980). With regard to the physical properties of sodium chloride, it is present either as colorless transparent crystals or as white crystalline powder, with a molecular weight of 58.44, melting point of 80˚C, boiling point of 1413˚C, pH of 6.7 to 7.3 and a density of 2.165 (Lewis, 1980). It is soluble in water and glycerine. One gram of sodium chloride will dissolve in 2.8 ml of water at 25˚C and a saturated solution will contain 26.5 g sodium chloride in 100 g of water (Shelef & Seiter, 1993). The solution is clear, colorless and odorless. It is stable under ordinary conditions of use and storage. Sodium constitutes 40% of sodium chloride by weight (Bodyfelt, 1982). To determine the salt content of a product, the food or its ash is extracted in warm water and the sodium and chloride contents determined by appropriate techniques. The concentration of sodium present in various bodily secretions can be measured through either flame photometry or by ion-specific electrodes (Michell, 1995). The chloride can be measured by titration using Morh’s or Volhards’s method (Luick, 1980). For assays of sodium chloride in various foods refer to ‘Official Methods of Analysis’ of the American Association of Analytical Chemists (1990).
III. ANTIMICROBIAL ACTIVITY The antimicrobial activity of sodium chloride may be called either direct or indirect depending upon the purpose it serves and the amount added in a food product (Sofos, 1983). In case of dried and smoked meats, a large amount of sodium chloride is added, which makes these products shelf stable. These products were popular in earlier days and in certain parts of the world. They depended solely on sodium chloride for their preservation, and hence the effect could be called direct. In recent years sodium chloride is added in minimal amounts and is combined with other preservatives or hurdles to prevent microbial growth. The amount of sodium chloride that needs to be added in foods required to prevent microbial growth is large (16.54% salt solution to bring the water activity to 0.90 (Robinson & Stokes, 1959)) and will cause an unacceptable taste and hence salt is usually combined with other preservation techniques. In certain instances, sodium chloride is
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added mainly as a flavoring and functional ingredient and hence in these cases the effect could be called indirect. In some fermented food products, sodium chloride in appropriate concentrations extracts nutrients from vegetables, which in turn allows the growth of lactic acid bacteria, thereby preventing growth of certain spoilage organisms and even pathogens such as Staphylococcus species. In these cases, the antimicrobial effect could be called indirect. Another reason that the antimicrobial effect of sodium chloride may be called indirect is that it reduces the water activity in many foods (Sperber, 1983) and thereby indirectly prevents microbial growth. The reduction in water activity of the food causes an osmotic shock to the bacterial cell. Plasmolysis occurs and the cell loses fluids and either dies or enters dormancy. Some other possible mechanisms of sodium chloride inhibition are limiting oxygen solubility to the microbial cell, alteration of pH, toxicity of sodium and chloride ions, loss of magnesium ions (Banwart, 1979) and interference with the cellular enzymes (Shelef & Seiter, 1993). Studies on the effect of sodium chloride on various organisms have indicated that sodium chloride could have a role on interfering with substrate utilization in these organisms. In Staphylococcus aureus sodium chloride was found to inhibit respiration, glucose utilization, phospho-β-galactosidase induction, and staphylococcal enterotoxin-A synthesis as well as hydrolysis of O-nitrophenyl-β-galactoside (ONPG), thereby inhibiting substrate transport into the bacterial cell (Smith et al., 1987). Erecinska and Deutsch (1985) studied the effect of sodium chloride on washed cells of Paracoccus denitrificans and found that increasing the concentration of sodium chloride (from 0.2 to 1.8%) gradually decreased the respiration rate and uptake of α-isoaminobutyrate with the highest concentration, completely inhibiting the uptake of the amino acid. In Clostridium sporogenes, glucose utilization was gradually inhibited and the level of intracellular ATP progressively decreased with increasing concentration of sodium chloride (Woods & Wood, 1982). However, the degree of glucose conversion to ethanol remained unchanged, indicating that sodium chloride interfered only with uptake and not with metabolism. In Pseudomonas fluorescens an increasing concentration of sodium chloride inhibited oxygen uptake (Prior, 1978). Protein synthesis was not always inhibited in different S. aureus cultures (Troller and Stinson, 1978). Bacteria can be classified into different groups based on their salt tolerance (Ayers et al., 1980). Those that grow well at concentrations ranging from 0 to 0.5% as well as tolerating higher levels are called nonhalophiles. Some bacteria belonging to the genera Staphylococcus, Micrococcus and Clostridium belong to this group. Those that can tolerate and grow in the range of 1.5 to 5.0% sodium chloride are called slight halophiles and some members of Achromobacter, Flavobacterium, Pseudomonas and Vibrio fall into this category. The third group, which includes those that can tolerate up to 5 to 20% sodium chloride, are called moderate halophiles. Some of the lactic acid bacteria and some spore formers fall under this category. Some of the moderate halophiles were studied for their susceptibility to a wide range of antibiotics at different salt concentrations and a group of them were found to have increased susceptibility at low salt concentrations (Coronado et al., 1995). Organisms that require and can grow in high concentrations of salt are called halophiles and those that can tolerate but not grow in high concentrations of salt are termed halodurics (Jay, 1992). The extreme halophiles require at least 9% sodium chloride for growth, with the optimum concentration for growth ranging between 12 to 23% and the maximum being 32% (Madigan et al., 1997). The cell wall of halophilic strain Halobacterium salinarum is stabilized by sodium ions, to such an extent that in low
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sodium environments or where the concentration of sodium is insufficient the cell wall breaks down causing cell lysis (Madigan et al., 1997). The need for sodium cannot be replaced by any other ion, including potassium. Obligate halophiles require and tolerate 15% sodium chloride and can be found in saturated brines. Bacteria that can grow in high salt concentrations however, are of less importance as food spoilage or pathogenic agents (Lueck, 1980). Sufficiently high amounts of sodium chloride are needed to cause bactericidal effects in foods and such amounts would not be permissible in foods, and such foods may not even be palatable. Hence, sodium chloride is generally used with other preservation methods. The antimicrobial effect of sodium chloride is thus dependent upon on several other factors present in foods as well as during food processing. Some of these factors include pH of the food, temperature and time during processing and storage, type of substrate, water activity of the substrate, type and populations of microorganisms, other preservatives/antimicrobial present in the substrate etc. Hence, most of the research done on sodium chloride is on its combinations with other hurdles and these studies will be discussed. As mentioned earlier, the mechanism of salt inhibition is by lowering the water activity of the substrate. Most of the pathogenic organisms will not grow below water activity of 0.90 to 0.92. One exception is Staphylococcus aureus, which has a generally recognized minimum water activity of 0.86, but has been reported to grow in conditions of water activity as low as 0.83 (Jay, 1992). This organism can grow in the presence of 7 to 10% sodium chloride with some strains being able to grow at 20% sodium chloride. Concentrations of sodium chloride up to 10% had very slight effects on the growth of S. aureus, but concentrations more than 3% caused a decline in the production of enterotoxin-B (McLean et al., 1968). In another study, both the cell growth and enterotoxin-B production were inhibited with increasing sodium concentration (0 to 5.3%), but there was no effect on enterotoxin-A production (Troller & Stinson, 1978). However, other researchers have shown an inhibitory effect of sodium chloride on enterotoxin-A production by S. aureus. Increasing the concentration from 0 to 4% (Pereira et al., 1982) and from 0 to about 10% (Smith et al., 1987) caused a decline in the enterotoxin-A production by the organism. An increase in the concentration of sodium chloride in tryptic soy broth caused an increase in the effectiveness of butylated hydroxyanisole (BHA) in inhibiting S. aureus. Accordingly, the strongest effect was observed at a combination of 100 ppm BHA and 5% or 10% sodium chloride (Stern et al., 1979). Sodium chloride (7%) exhibited a synergistic effect with potassium sorbate (0.2%) in inhibiting S. aureus strains in TSB at 37oC (Robach & Stateler, 1980). However, there was no synergistic effect of sodium chloride (2, 3 and 7%) and potassium sorbate (0.2 and 0.3%) observed after prolonged exposure (15 days at 22oC and 48 h at 35oC) (LaRocco & Martin, 1987). An alternative sigma factor s B, produced by S. aureus as a response to environmental stresses was repressed in the presence of 1 M sodium chloride (Chan et al., 1998). There are reports in the literature showing that the heat resistance of S. aureus increases with increasing concentrations of sodium chloride due to a decrease in the water activity of the medium. Sodium chloride at different concentrations (3, 5 and 9 % w/v ) protected S. aureus from heat injury, with the highest concentration affording the maximum protection (Smith et al., 1982). The authors suggested that sodium chloride might be involved in stabilizing membrane protein structures such as nucleic acids and nucleotides as well as increasing the melting temperatures of membrane phospholipids.
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Thus, the damage to the cell membrane and leakage of cell components from the cytoplasm is prevented. In another study, 4 and 8% sodium chloride protected S. aureus cells from heat injury at pH 7.0 while at pH 6.5 a concentration of 8% gave protection (Bean & Roberts, 1975). Different substrates with reduced water activity were inoculated with S. aureus and the organism showed increased heat resistance (Troller, 1973). The effects of salt on thermal resistance have been examined by determining the relationships between thermal resistance and either solute concentration or water activity of the heating menstruum (Juneja et al., 1999). The heat resistance of S. aureus in sodium chloride increased as the degree of salt-water association increased (Tuncan & Martin, 1990). The authors explained that the effects of salt on thermal inactivation of microorganisms are mainly related to reduced water activity and increased osmotic pressure of the heating menstruum. For a given solute a certain optimum concentration of the solute gives a maximum heat protection, whereas levels outside this optimum solute concentration result in an increase in the heat sensitivity of the organism (Leistner & Russell, 1991). The influence of sodium chloride on spore formers has been the subject of interest for many researchers. Sodium chloride has been found to inhibit toxin production in Clostridium botulinum. Greenberg et al. (1959) studied the inhibitory effect of sodium chloride on growth and toxin production in C. botulinum types A and B in cured meat. With less than 6.25% sodium chloride there was no inhibition of toxin production as well as putrefactive changes. Between 6.25 and 9% there was no inhibition on toxin production but the putrefactive changes did not occur. Above 9% growth was inhibited. In laboratory medium, 3 to 4 % sodium chloride inhibited toxin production by C. botulinum type E (Segner et al., 1966). The influence of sodium chloride on toxin production by C. botulinum types A, B and C at different temperatures in cooked meats vacuum packed in airimpermeable plastic pouches was studied (Pivnick & Barnett, 1965). Toxin production in both types was inhibited by 3% salt during 4 weeks at 30˚C. However, 2.2% salt did not inhibit toxin production at 30˚C in 1 week, while it did in 1-month at 25oC and in 2 months duration at 20˚C. Sodium chloride at concentrations 2.1 and 3.4% inhibited toxin production in cooked ham within a month at 15˚C. In the case of C. botulinum type E, 1.9% sodium chloride failed to inhibit toxin production in jellied pork tongue, while 2.7% sodium chloride was very effective in inhibiting toxin production. The authors suggested adequate refrigeration and an increase in salt concentration to acceptable limits for types A and B and heat and low salt concentration for type E. Sodium chloride at 1.4 and 2.3% concentrations did not inhibit toxin production by C. botulinum E in jellied ox tongue (Pivnick & Bird, 1965). A concentration of 5.0% sodium chloride at pH values lower than 5.03 was needed to inhibit growth of C. botulinum type E (Segner et al., 1966). The effect of sodium chloride on growth of C. botulinum spores at different temperatures and pH levels in the presence of sodium nitrite was investigated (Emodi & Lechowich, 1969). The substrate was laboratory media and the pH range varied from 5.2 to 6.6. About 4.87% sodium chloride was sufficient to inhibit outgrowth at all temperatures (30, 15.6, 10, 7.2, 5.0 and 3.4) with lower temperatures requiring slightly lower concentrations. At lower temperatures, inhibition occurred at high pH levels. In bottled lumpfish caviar toxin production of C. botulinum was inhibited at combinations of sodium chloride concentrations >5.56% and pH 42 gm/m3/1H1 (J. T. Baker, Material safety data sheet, 1996). The same reference cites LD50 for rabbits via skin to be >10 gm/kg and estimated it to be a mutagen and terratogen. For a detailed toxicity data and safety profile, refer to a food safety additives handbook. About 1 to 3.3 g/day is the level of sodium that is considered safe as well as adequate for the body (Darby, 1980). Owing to its solubility in water, salt is excreted relatively easily and quickly from the body through the kidneys as well as the skin (in the form of sweat). Renal losses are about 6.0 to 12.5 g/day (Darby, 1980). The effect of sodium chloride on cell division of rats was studied (Lugli & Lutz, 1999). Sodium chloride was given as a supplement at 2 and 4% concentrations in the feed for 4 weeks. This feed resulted in a significant stimulation of cell division in the stomach and liver with both concentrations of sodium chloride and in the bladder with 4% sodium chloride. Feed with ascorbic acid (2g/kg feed) or β-carotene (12.5 mg/kg feed) for 1 week before sodium chloride supplementation inhibited the stimulation of cell division.
VII. SUMMARY Sodium chloride, commonly called table salt or salt, is a vital part of human life. Salt enhances the flavor of foods and plays a preservative as well as functional role in food processing. Apart from its use in the food industry, salt has uses in the agricultural and chemical industries as well as in water conditioning and transportation. Sodium chloride has been designated the fifth element and is abundantly available in nature. The production and recovery methods of sodium chloride are described. Two elemental substances, the cationic sodium and the anionic chloride, react to form the halide salt ‘sodium chlo-
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ride’. Sodium chloride occurs in the form of colorless transparent crystals or white crystalline powder, with a molecular weight of 58.44. To determine the salt content of a food product, the food or its ash is extracted in warm water and the sodium and chloride contents determined by appropriate techniques. The antimicrobial activity of salt can be both direct or indirect depending on the amount added and the purpose it serves. Since the amount of sodium chloride needed to be added to foods to prevent microbial growth is large and will cause an unacceptable taste, it is usually added in combination with other hurdles. The mechanism of inhibition of microorganisms by sodium chloride is mainly by lowering the water activity of the substrate. Studies have also indicated that sodium chloride could have a role in interfering with substrate utilization in microorganisms. The influence of sodium chloride alone as well as its interactive effects with other factors on various microorganisms such as Staphylococcus aureus, spore formers, Escherichia coli O157:H7, Listeria monocytogenes etc. in laboratory media as well as foods has been discussed in detail. The effect of sodium chloride on the heat resistance of microorganisms is discussed as well. The functional applications of sodium chloride in various products are discussed. Excessive sodium intake in humans has been linked to hypertension and the related cardiovascular problems and stroke. Hence there are many consumer concerns and the food industry is trying to minimize the salt content of food products.
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Allen, A. E. Jr., and Day, J. W. 1980. Low sodium salt seasoning. U. S. Patent. 4,216,244. August, 5. Askar, A., El-Samahy, S. K., Shehata, H. A., and Tawfik, M. 1993. Pasterma and beef bouillon. The effect of substituting KCl and K-lactate for sodium chloride. Fleischwirtschaft. 73:289-292. Ayres, J. C., Mundt, J. O., and Sandine, W. E. 1980. Microbiology of Foods. San Francisco: W. H. Freeman and Company. Baker, J. T. 1996. Material Safety Data Sheet on sodium chloride. Banwart, G. J. 1979. Basic Food Microbiology. Connecticut: AVI Publishers. Bean, P. G., and Roberts, T. A. 1975. Effect of sodium chloride and sodium nitrite on the heat resistance of Staphylococcus aureus NCTC 10652 in buffer and meat macerate. J. Food Technol. 10:327-332. Bello-Perez, L. A., and Paredes-Lopez, O. 1996. Starch and amylopectin- Effects of solutes on clarity of pastes. Starch. 48:205-207. Bodyfelt, F. W. 1982. Processors should put some pinch on salt. Dairy Rec. 82:83-84. Boyd, E. M., and Boyd, C. E. 1973. Toxicity of Pure Foods. Cleveland: CRC Press. Breierova, E. 1997. Yeast exoglycoproteins produced under NaCl-stress conditions as efficient cryoprotective agents. Lett. Appl. Microbiol. 25:254-256. Briggs, A., and Yazdany, S. 1970. Effect of sodium chloride on the heat and radiation resistance and on the recovery of heated or irradiated spores of the genus Bacillus. J. Appl. Bacteriol. 33:621-632. Buchanan, R. L., and Golden. M. H. 1995. Model for the non-thermal inactivation of Listeria monocytogenes in a reduced oxygen environment. Food Microbiol. 12:203-212. Buchanan, R. L., Golden. M. H., and Phillips, J. G. 1997. Expanded models for the thermal inactivation of Listeria monocytogenes. J. Appl. Microbiol. 82:567-577. Buchanan, R. L., Stahl, H. G., and Whiting, R. C. 1989. Effects and interactions of temperature, pH, atmosphere, sodium chloride and sodium nitrite on the growth of Listeria monocytogenes. J. Food Prot. 52:844851. Buckenhuskes, H. J. 1997. Fermented vegetables. In Food Microbiology- Fundamentals and Frontiers, ed. M. P. Doyle, L. R. Beuchat and T. J. Montville, pp 600-601. Washington, D. C.: ASM Press. Chan, P. F., Foster, S. J., Ingham, E., and Clements, M. O. 1998. The Staphylococcus aureus alternative sigma factor sB controls the environmental stress response but not starvation survival or pathogenicity in a mouse abscess model. J. Bacteriol. 180:6082-6089. Cheville, A. M., Arnold, K. W., Buchrieser, Cheng, C.-M., and Kaspar, C. W. 1996. rpoS regulation of acid, heat and salt tolerance in Escherichia coli O157:H7. Appl. Environ. Microbiol. 62:1822-1824.
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Okai, H., Tamura, M., Seki, T., Tada, M., and Kawasaki, Y. 1989. An enhanced effect of sodium chloride using amino acid esters and amino acids. Chem. Senses. 14:320. Pagan, R., Condon, S., and Sala, F. J. 1997. Effects of several factors on the heat shock-induced thermotolerance of Listeria monocytogenes. Appl. Environ. Microbiol. 63:3225-3232. Paul, A. A., and Southgate, D. 1978. In: McCance and Widowson’s -Composition of Foods. H. M. S. O. Pastoriza, L., Sampedro, G., Herrera, J. J., and Cabo, M. L. 1998. Influence of sodium chloride and modified atmosphere packaging on microbiological, chemical and sensorial properties in ice storage of slices of hake (Merluccius merluccius). Food Chem. 61:23-28. Pearson, A. M., and Wolzak, A. M. 1982. Salt- its use in animal products, a human health dilemma. J. Animal Sci. 54:1263-1278. Pereira, J. L., Salzberg, S. P., and Bergdoll, M. S. 1982. Effect of temperature, pH and sodium chloride concentrations on production of staphylococcal enterotoxin A and B. J. Food Prot. 45:1306-1309. Pivnick, H., and Barnett, H. 1965. Effect of salt and temperature on toxinogenesis by Clostridium botulinum in perishable cooked meats vacuum-packed in air-impermeable plastic pouches. Food Technol. 142:1164-1167. Pivnick, H., and Bird, H. 1965. Toxinogenesis by Clostridium botulinum types A and E in perishable cooked meats vacuum-packed in plastic pouches. Food Technol. 19:132-140. Pivnick, H., and Thacker, C. 1970. Effect of sodium chloride and pH in initiation of growth by heat-damaged spores of Clostridium botulinum. Can. Inst. Food Technol. J. 3:70-75. Prior, B. A. 1978. The effect of water activity on growth and respiration of Pseudomonos fluorescens. J. Appl. Microbiol. 4:97-106. Razavi-Rohani, S. M., and Griffiths, M. W. 1996. Inhibition of spoilage and pathogenic bacteria associated with foods by combinations of antimicrobial agents. J. Food Safety 16:87-104. Reddy K. A., and Marth, E. H. 1991. Reducing the sodium content of foods: A review. J. Food Prot. 54: 138-150. Robach, M.C., and Stateler, C. L. 1980. Inhibition of Staphylococcus aureus by potassium sorbate in combination with sodium chloride, tertiary butylhydroquinone, butylated hydroxyanisole or ethylenediamine tetraacetic acid. J. Food Prot. 43:208-211. Roberts, T. A., Gilbert, R. J., and Ingram, M. 1966. The effect of sodium chloride on heat resistance and recovery of heated spores of Clostridium sporogenes (PA 3679/S2). J. Appl. Bacteriol. 29:549-555. Robinson, R. A., and Stokes, R. H. 1959. Electrolyte Solutions. The Measurement and Interpretation of Conductance, Chemical Potential and Diffusion in Solutions of Simple Electrolytes. London: Butterworths. Salt Institute, 1999. History of salt. Internet website publication. Sasaki, M. 1996. Influence of sodium chloride on the levels of flavor compounds produced by Shoyu yeast. J. Agric. Food Chem. 44:3273-3275. Sathe, S. K., Deshpande, S. S., and Salunkhe, D. K. 1984. Dry beans of Phaseolus. A review. Part 1. Chemical composition:proteins. CRC Crit. Rev. Food Sci. Nutr. 20:1-46. Sathe, S. K., Idouraine, A., and Weber, C. W. 1994. Purification and biochemical characterization of tepary bean (Phaseolus acutifolius) major globulin. Food Chem. 50:261. Sathe, S. K., and Sze-tao, K. W. C. 1997. Effects of sodium chloride, phytate and tannin on in vitro proteolysis of phaseolin. Food Chem. 59:253-259. Schreiber, B. C., and Harner, H. L. 19. Sixth international symposium on salt. Vol 2. Virginia: The Salt Institute. Segner, W. P., Schmidt, C. F., and Boltz, J. K. 1966. Effect of sodium chloride and pH on outgrowth of spores of type E Clostridum botulinum at optimal and suboptimal temperatures. Appl. Microbiol. 14:4954. Seman, D. L., Olson, D. G., and Mandigo, R. W. 1980. Effect of reduction and partial replacement of sodium on bologna characteristics and acceptability. J. Food Sci. 45:1116-1121. Shackelford, J. R. 1981. Salt substitutes having reduced bitterness. U. S. Patent. 4,297,375. Oct, 27. Shelef, L. A., and Seiter, J. A. 1993. Indirect antimicrobial. In Antimicrobial in Foods, ed. P. M. Davidson and A. L. Branen. pp. 539-569. New York: Marcel Dekker. Smith, J. L. Benedict, R. C.,and Palumbo, S. A. 1982. Protection against heat-injury in Staphylococcus aureus by solutes. J. Food Prot. 45:54-58. Smith, J. L., and Hunter, S. E. 1988. Heat injury in Listeria monocytogenes. Prevention by solutes. Lebensm. Wiss. Technol. 21:307-311. Smith, J. L., Maurer, M. J., Bencivengo, M. M., and Kunsch, C. A. 1987. Effect of sodium chloride on uptake of substrate by Staphylococcus aureus 196E. J. Food Prot. 50:968-974.
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123. Sofos, J. N. 1983. Antimicrobial effects of sodium and other ions in foods: A review. J. Food Safety. 6: 4578. 124. Sperber, W. H. 1983. Influences of water activity on foodborne bacteria: a review. J. Food Prot. 46:142150. 125. Stern, N. J., Smoot, L. A., and Pierson, M. D. 1979. Inhibition of Staphylococcus aureus growth by combinations of butylated hydroxyanisole, sodium chloride and pH. J. Food Sci. 44:710-712. 126. Sternberg, M., Cornelius, D. A., Eberts, N. J., Schwende, F. J., and Chiang, J. P. C. 1980. Glycinamide hydrochloride, a compound with common salt flavor. In Biological and Behavioral Aspects of Salt Intake, ed M. R. Kare, M. J. Fregly and R. A. Bernard, pp 319-329. New York: Academic Press. 127. Stringer, S. C., and Peck, M. W. 1997. Combinations of heat treatment and sodium chloride that prevent growth from spores of nonproteolytic Clostridium botulinum. J. Food Prot. 60:1553-1559. 128. Sutherland, J. P., Bayliss, A. J., and Braxton, D. S. 1995. Predictive modeling of growth of Escherichia coli O157:H7. The effects of temperature, pH and sodium chloride. Int. J. Food Microbiol. 25:29-49. 129. Tada, M., Shinoda, I., and Okai, H. 1984. L-Ornithyltaurine, a new salty peptide. J. Ag. Food Chem. 32:992-996. 130. Telis, V. R. N., and Kieckbusch, T. G. 1998. Viscoelasticity of frozen/thawed egg yolk as affected by salts, sucrose and glycerol. J. Food Sci. 63:20-24. 131. Terrell, R. N. 1983. Reducing the sodium content of processed meats. Food Technol. 37:66-71. 132. Tomicka, A., Chen, J., Barbut, S., and Griffiths, M. W. 1997. Survival of bioluminescent Escherichia coli O157:H7 in a model system representing fermented sausage production. J. Food Prot. 60:1487-1492. 133. Troller, J. A. 1973. The water relations of foodborne bacterial pathogens: a review. J. Milk Food Technol. 36:276-288. 134. Troller, J. A., and Stinson, J. V. 1978. Influence of water activity on the production of extracellular enzymes by Staphylococcus aureus. Appl. Environ. Microbiol. 35:521-526. 135. Tuncan, E. U., and Martin, S. E. 1990. Combined effects of salts and temperature on the thermal destruction of Staphylococcus aureus MF-31. J. Food Sci. 55:833-836. 136. Valero, E., and Garcia-Carmona, F. 1998. pH-dependant effect of sodium chloride on latent grape polyphenol oxidase. J. Agric. Food Chem. 46:2447-2451. 137. Volker, U., Mach, H., Schmid, R., and Hecker, M. 1992. Stress proteins and cross-protection by heat shock and salt stress in Bacillus subtilis. J. Gen. Microbiol. 138:2125-2135. 138. Wang, D., Tang, J., Correia, L. R. and Gill, T. A. 1998. Postmortem changes of cultivated Atlantic salmon and their effects on salt uptake. J. Food Sci. 63:634-637. 139. Woods, L. F. J., and Wood, J. M. 1982. The mechanism of the inhibition of Clostridium sporogenes by sodium chloride. British Food Manufacturing Industries Research Assn. Research Report. No. 382. 140. Zaika, L. L., Engel, L. S., Kim, A. H., and Palumbo, S. A. 1989. Effect of sodium chloride, pH and temperature on growth of Shigella flexneri. J. Food Prot. 52:356-359.
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A. Prakash
Polyphosphates
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I. INTRODUCTION Phosphorus, as the phosphate anion, is essential to sustain life. It is a component of many enzyme systems involved in the metabolism of various nutrients, and the formation and structure of various tissues (Ellinger, 1972). Thus, phosphates are natural constituents of almost every food we eat. To produce food grade phosphates, mined phosphates are converted to phosphoric acid, followed by partial or complete neutralization with alkalis such as sodium, potassium, or calcium. Their buffering capacity, ability to sequester metal ions, water-holding capacity, and ability to interact with long chain polyelectrolytes such as protein, make phosphates widely used as food additives. The classification, and various applications of polyphosphates in food products are summarized in TABLE 1. Corresponding chemical structures are shown in FIGURE 1. Inclusion of polyphosphates as functional additives in many food formulations and observations of preservative activity have prompted researchers to elucidate the mechanism of antimicrobial action. Regardless, polyphosphates continue to be added to foods as functional additives, with their antimicrobial effect being regarded as an added benefit rather than their primary function. The only approved antimicrobial use of an orthophosphate is in a prechill or post-chill dip to reduce microbial levels of raw poultry carcasses.
II. STRUCTURE/CHEMISTRY Phosphates are derived from phosphoric acid neutralized with alkali metal ions, such as sodium, potassium, or calcium. There are two classes of phosphates: orthophosphates and condensed phosphates. Orthophosphates, prepared from orthophosphoric acid, H3PO4, consist of a phosphorus atom surrounded by four oxygens. This molecule has three replaceable hydrogen molecules giving rise to a number of combinations of hydrogen and metal cations such as monobasic orthophosphates (one alkali metal ion and two hydrogen molecules), dibasic orthophosphates (two alkali metal ions and one hydrogen), and tribasic orthophosphates (three metal ions). Orthophosphates when heated (a process © 2000 by CRC Press LLC
pH1
Solubility2
ORTHOPHOSPHATES
Monosodium phosphate Disodium phosphate Disodium phosphate dihydrate Trisodium phosphate Monopotassium phosphate Dipotassium phosphate Tripotassium phosphate Monocalcium phosphate
NaH2PO4 Na2HPO4 Na2HPO4 2H2O Na3PO4 KH2PO4 K2HPO4 K3PO4 Ca(H2PO4)2 H2O
4.6 9.2 0.9 11.8 4.6 9.3 11.9 3.8
87 12 15 14 25 168 107
Emulsifier, buffer Emulsifier, buffer Emulsifier, buffer Emulsifier, buffer Water binding in meats Emulsifier, buffer Emulsifier, buffer Acidulant, leavening acid, dough conditioner, yeast food, nutrient
Sodium acid pyrophosphate
Na2H2P2O7
4.3
15
Tetrasodium pyrophosphate
Na4P2O7
10
3.8
Tetrapotassium pyrophosphate
K4P2O7
10.5
187
Sodium tripolyphosphate Potassium tripolyphosphate Sodium polyphosphates, glassy, or Graham’s Salt; three chain lengths; sodium hexametaphosphate has an average chain length of 13 Sodium trimetaphosphate Sodium tetrametaphosphate
Na5P3O10 K5P3O10 (NaPO3)13Na2O (NaPO)21Na2O (NaPO)5 Na2O
9.9 9.6 7.7 6.9 6.3
15 193 40
Emulsifier, buffer, sequestrant, water binding agent in meats Dispersant, coagulant, crystallization inhibitor in canned tuna Emulsifier, water binding agent in meats, suspending agent Emulsifier, water binding agent in meats Emulsifier, water binding agent in meats Sequestrant, emulsifier, water binding agent in meats, suspending agent
(NaPO3)3 (NaPO3)4 4H2O
6.7 6.2
23 18
CONDENSED PHOSPHATES Pyrophosphates
Tripolyphosphates Long-chain polyphosphates
Metaphosphates
1 pH
measurement represents a 1% solution; 2 Solubility measurement at 25°C (g/100g water)
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Functions
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Formula
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TABLE 1: Classes, Formulas, pH, Solubility, and Functions of Several Phosphates
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FIGURE 1. Stereochemical structures of various polyphosphates
called calcining), condense to form straight chain compounds (polyphosphates) and cyclic compounds (metaphosphates). Straight chain compounds consist of pyrophosphates with two monomers, tripolyphosphates with three orthophosphates, and polyphosphates with four or more orthophosphates. While the pyrophosphates and tripolyphosphates are crystalline materials, the straight chain polyphosphates form amorphous or glassy particles. The cyclic metaphosphates are not commonly used in the food industry, although sodium trimetaphosphate is approved by the FDA for modification of food starches. Another seldom used form is referred to as ultraphosphates, which incorporate branching PO4 groups in the structure resulting in branched chains and rings as well as combinations of chains and rings. Branched phosphates rapidly hydrolyze to structures with no branching points (Van Wazer, 1971). A. Properties Orthophosphates have a pH range of 4.0-12.0, thus considered to be compounds with superior buffering capacity (Prasad & Prasad, 1989). They are also used in foods to adjust pH to optimum values. While pyrophosphates are good buffers in the pH range (5.5-7.5) of most foods longer chain polyphosphates are less effective (Sofos, 1989). Long chain polyphosphates are polyelectrolytes and react with other polyelectrolytes such © 2000 by CRC Press LLC
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as proteins, pectins, and starches to function as dispersive and emulsifying agents. They can form strong complexes with metal ions such as calcium and magnesium; higher pH increases such complexing efficiency. Short-chain polyphosphates can efficiently sequester heavy metal ions such as iron and copper, in this case, increasing pH decreases complexing efficiency. Ring phosphates form weaker complexes with cations and orthophosphates form complexes only at very low concentrations and precipitates at higher concentrations. (Wagner, 1986). The ability to sequester metal ions (form soluble complexes) is the basis of the mechanism of antimicrobial action. B. Assay The level of orthophosphate obtained from hydrolysis of polyphosphates can be determined by a colorimetric method. This method is based on the rapid formation of molybdenum blue color by the reaction of orthophosphate with molybdenum ions in the presence of ascorbic acid-trichloroacetic acid and citrate-arsenite reagents (Murphy & Riley, 1962; Dick & Tabatabai, 1977). NMR and gel filtration have been used to calculate the average length of polyphosphate chains (Wood & Clark, 1988). Tsuji et al. (1994) and Yasuno et al. (1996) determined the orthophosphate content in various raw and processed foods by ion chromatography. A modified thin-layer chromatographic (TLC) method for condensed polyphosphate determination in frozen seafood is described by Krzynowek and Panunzio (1995).
III. ANTIMICROBIAL ACTIVITY A. Mechanism(s) A number of mechanisms for the antimicrobial activity of polyphosphates have been suggested. The foremost mechanism suggested is the chelation of metal ions in cell membranes which leads to cation deficiency with resulting loss of membrane integrity and inhibition of normal cell division (Wagner, 1986). Other mechanisms include effect of pH (Shelef et al., 1990), increase in ionic strength, interactions with cell walls and membranes (Kohl, 1971), and interference with various transport functions (Knabel et al., 1991). Polyphosphates can form stable complexes with metallic ions thus preventing precipitation or redissolving precipitates of alkaline earth metals (Van Wazer & Callis, 1958). Cobalt, copper, and iron are bound strongly by polyphosphates while calcium and magnesium are less strongly bound; these bound ions then become unavailable for metabolic functions. Because polyphosphates are polyvalent anions, they have a high degree of surface activity causing them to aggregate at cell surfaces when dissolved in water. Microbial cell membranes contain metal chelators, which are responsible for ferrying metal ions across the membrane. Metal chelating agents such as polyphosphates may compete with cell membrane-chelators for available ions and selectively remove calcium and magnesium or other ions from the cell wall, membranes, or cytoplasm. Post et al. (1968), suggested that this mechanism accounts for the observed lysis of gram-negative bacteria and the growth inhibition of gram-positive bacteria as well as fungi. Seward et al. (1982), examined the germination of C. botulinum type E spores in media supplemented with several antibotulinum agents, including sodium hypophosphite and sodium tripolyphosphate. At high pH levels, 0.5 or 1.0% hypophosphite and the combination of 1.5% potassium sorbate and 0.5% sodium tripolyphosphate resulted in germination and © 2000 by CRC Press LLC
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outgrowth of abnormally shaped cells culminating in cell lysis and defective cell division. Support for the metal chelation theory is provided by the fact that in foods that contain higher concentrations of divalent cations, polyphosphates are not as effective as in culture media (Shelef et al., 1990; Rajkowski, 1994; Zaika et al., 1997). Knabel et al. (1991), also showed that orthophosphates that lack the metal chelating potential did not inhibit Aspergillus flavus or any of the several gram-positive as well as gram-negative bacteria tested. Molins and co-workers (1987) reported that bacterial inhibition did not correlate with soluble orthophosphate content in ground pork. Addition of free cations to polyphosphate-containing cultures has been shown to reverse the inhibitory effects of polyphosphates on bacterial growth (Elliott et al., 1964; Jen & Shelef, 1986; Knabel et al., 1991). Knabel et al. (1991) sought to explain the difference in inhibition of polyphosphates on growth of gram-negative versus gram-positive bacteria. Walls of most grampositive bacteria consist of a thick layer of peptidoglycan and large amounts of teichoic and/or teichuronic acids. These anionic polymers can bind metal ions and are responsible for maintaining a high concentration of bivalent cations such as Ca2+, Mg2+, Mn2+, and Fe3+for cation-dependent membrane systems. Polyphosphates are able to remove metal ions from the cell membranes because of their higher affinity for the metal cations, thus inhibiting growth. Because gram-negative bacteria have more efficient systems for binding and transporting metal ions across cell membranes, polyphosphates are not as successful in chelating the metal ions, and thus not as effective in inhibiting gram-negative bacteria. The authors also suggested that fungi are inhibited by polyphosphates due to polymers such as chitin, chitosan, and glycoproteins present in their cell walls and which are involved in the passive uptake of metals. Working with pure cultures of Staphylococcus aureus, Lee et al. (1994a) attributed the antibacterial effects of polyphosphates to damage to the cell wall or cell membrane which resulted in the leakage of intracellular nucleotides and proteins. The addition of Ca2+ and Mg2+ reversed the bactericidal and bacteriolytic effects (Lee et al., 1994b). It was also determined that polyphosphates bound to cell walls did not release metals from the cell walls into the medium leading to the conclusion that polyphosphates remain bound to the cell walls even after chelating metal ions from the cell walls (Lee et al., 1994c). The authors offered the hypothesis that structurally essential metals such as magnesium form bridges across phosphate groups in adjacent ribitol teichoic acid chains in S. aureus cell walls and that polyphosphates bound to the cell walls chelate these metals resulting in bactericidal and bacteriolytic effects. Matsuoka et al. (1995), suggested that the antibacterial action of sodium hexametaphosphate on S. aureus was caused by a weak effect on cell membranes resulting in loss of osmoregulation and selective permeability due to damage to the membrane, as well as loss of metabolic function caused by substrate leakage. Other researchers have proposed that enzyme inhibition may be responsible for the antimicrobial mechanism. Wagner and Busta (1985) found that sodium acid pyrophosphate (SAPP) in culture media inhibited the production or activity of the protease responsible for activating C. botulinum toxin resulting in delayed toxigenicity in meat formulations inoculated with C. botulinum. Using fish muscle, Tarr (1951) showed that SAPP inhibited 5’-nucleotidase which hydrolyses adenosine monophosphate (AMP) to adenosine and orthophosphate thus demonstrating that inorganic pyrophosphates can regulate enzyme activity. In the previous year, Vishniac (1950) investigated the effect of sodium tripolyphosphate on yeast hexokinase, and reported that the compound inhibited © 2000 by CRC Press LLC
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the anaerobic conversion of glucose by intact yeast cells, yeast zymase preparations, as well as crystalline hexokinase preparations and that the inhibition was reversed by addition of ATP. It was concluded that polyphosphate inhibition was due to chelation of Mg2+, which is essential for hexokinase activity and that ATP competes with polyphosphate for the metal ions. B. Spectrum The following is a review of studies published in the past ten years. Prior studies have been reviewed by Tompkin, 1984; Wagner, 1986; Sofos, 1989; Molins, 1991 and Shelef & Seiter, 1993. In the eighties there was particular emphasis on the effect of polyphosphates on C. botulinum and S. aureus growth and toxin production in culture media as well as cured and restructured meat products. The emergence of pathogens such as Salmonella, E. coli O157:H7, and Listeria monocytogenes, has prompted recent investigations into the suppression of growth of these bacteria by polyphosphates. 1. Clostridia: Pasteurized process cheese spread containing one of three types of phosphate emulsifiers was inoculated with Clostridium botulinum and analyzed over 30 weeks for growth of C. botulinum and toxigenesis (Eckner et al., 1994). Toxin formation was observed at 8 weeks in the 60% moisture cheese containing disodium orthophosphate, while the polyphosphates containing cheeses tested positive for toxin at 20 weeks. Toxin formation did not occur in cheese spreads with lower moisture containing phosphates. The results indicate that polyphosphates in high moisture cheese spreads can impart a margin of safety by delaying toxin formation, although toxigenesis is not prevented. Loessner et al. (1997) investigated the effects of polyphosphates on the growth and development of C. tyrobutyricum in processed cheese spreads. Butyric blowing is a common defect observed in such products caused by outgrowth of C. tyrobutyricum spores. They found that 0.5% sodium polyphosphate glassy was sufficient to control C. tyrobutyricum growth under normal conditions, while 1% totally inhibited the organism. 2. Staphyloccocus aureus: At pH 7.0, 1.2% sodium acid pyrophosphate (SAPP), 1% sodium tripolyphosphate (STPP), or 0.4% sodium hexametaphosphate (also known as sodium polyphosphate, glassy or SPG) exhibited no antibacterial action against S. aureus strain 196E in N-Z amine broth plus 1% yeast extract (Shelef & Wang, 1989), although a bacteriostatic effect was observed at slightly higher concentrations. Without pH adjustment, 1% SAPP decreased the pH of the media to 5.5 at which level significant inhibition of the bacterium was observed. In contrast, 1% SAPP in BHI broth (pH 6.0) did not significantly inhibit S. aureus, whereas alkaline phosphates (pH 7.8) exhibited higher antimicrobial effectiveness (Knabel et al., 1991). Lee et al. (1994a) compared the effects of different phosphates on the growth of S. aureus ISP40 8325 in a synthetic medium. The minimum inhibitory concentrations were found to be 0.1% for sodium ultraphosphate and sodium polyphosphate glassy and 0.5% for SAPP and tetrasodium pyrophosphate (TSPP), indicating that long chain polyphosphates exerted greater inhibition (FIGURE 2). Addition of 1% SAPP to custard reduced counts of S. aureus strain 196E by about 0.5 log, and in beef, 0.5 and 1.0% SAPP reduced counts by 1.5-2 logs at 22°C (Shelef et al., 1990). This effect was eliminated when pH was adjusted to that of the control or when the storage temperature was increased to 30°C. When the pH of beef was adjusted to the same levels as produced by 0.5 and 1.0% SAPP, no significant differences © 2000 by CRC Press LLC
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FIGURE 2. Effect of phosphates at MIC on growth (mean log CFU/ml) of early-exponential-phase cells of Staphylococcus aureus (redrawn from Lee et al., 1994a).
between the treatments was apparent. The authors surmised that the reduction of pH due to SAPP addition was a major factor in the observed growth inhibition. STP and SHMP had no effect on bacterial growth. Likewise, addition of 0.5 or 1.0% SHMP to UHT-sterilized milk had no activity against S. aureus 196E at 19, 28, and 37°C (Rajkowski et al., 1994), although SHMP enhanced the inhibitory effect of NaCl. The high levels of Ca2+ and Mg2+ in custard (Shelef et al., 1990) as well as UHT milk (Rajkowski et al., 1994) were most likely responsible for elimination of the inhibitory effects of polyphosphate. It appears that SAPP compared to other phosphates has a greater inhibitory effect on S. aureus in food, although the inhibition is small. The inhibition seems to be related to the decrease in pH by SAPP and is enhanced in the presence of other antimicrobials. 3. Listeria monocytogenes: While SAPP appears to be most effective against S. aureus, the higher polymers are more effective in inhibiting growth of L. monocytogenes. The effect of three sodium polyphosphate polymers (average chain lengths = 6, 13, and 21) on the growth of L. monocytogenes in BHI containing 0.3% glucose, pH 6.0 at 28, 19, 10 and 5°C were evaluated (Zaika & Kim, 1993). The longer polymers were more inhibitory. Higher concentrations, lower temperatures, decreasing pH, as well as addition of NaCl enhanced the inhibitory effect (Zaika et al., 1997). Growth inhibition was reversed by addition of certain polyvalent metal cations, especially Ca2+, Mg2+, and Mn2+. Thus, in foods with high levels of metal cations such as UHT-sterilized milk and singleingredient baby foods, sodium polyphosphate exerted little or no inhibition on the growth of L. monocytogenes (Rajkowski et al., 1994; Zaika et al., 1997). Knabel et al. (1991) found that suppression of L. monocytogenes by 1% tetrasodium pyrophosphate (TSPP) could be reversed by iron supplementation. Addition of a 0.5% commercial phosphate blend to smoked sausage and cured smoked ham inoculated with L. monocytogenes had minimal or no effect (Flores et al., 1996).
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Surface disinfection of chicken skin inoculated with L. monocytogenes with 1% trisodium phosphate (TSP) was more effective than solutions of 10% monosodium phosphate (MSP), SAPP, SPG, and STPP (Hwang & Buechat, 1995). Addition of Tween 80 to TSP did not enhance removal of Listeria. 4. Salmonella: In general, gram-negative bacteria are less inhibited by phosphates than are gram-positive bacteria. Nevertheless, the effectiveness of polyphosphates in inhibiting the growth of Salmonella in egg whites, chicken breast muscle, and culture media, has been demonstrated (Garibaldi et al., 1969; Foster & Mead, 1976; Molins et al., 1984). Tetrasodium pyrophosphate (TSPP) in BHI broth inhibited growth of S. typhimurium, and addition of Fe3+ enhanced the inhibition (Knabel et al., 1991). The authors theorized that formation of the polyphosphate-iron chelate complex blocked siderophore receptors on the surface of the cells preventing siderophore-mediated Fe3+ transport. In 1992, the U.S. Department of Agriculture approved the use of trisodium phosphate (TSP) as a postchill processing aid to remove bacteria from the surfaces of raw poultry carcasses (Geise, 1993). It is hypothesized that TSP enables the removal of a thin layer of fat on the surface of poultry skin allowing the removal of bacteria embedded in the tissue (Geise, 1994). Two patents describe the reduction in counts in broiler carcasses inoculated with nalidixic acid-resistant (NAL) Salmonella typhimurium with a 10% TSP postchill dip (Bender & Brotsky, 1991; Bender & Brotsky, 1992). Kim & Slavik, 1994 achieved a 2-log reduction on salmonella inoculated chickens by treating with TSP. A 1% TSP was significantly more effective than solutions of 10% monosodium phosphate (MSP), SAPP, SPG, and STPP in reducing the levels of Salmonella spp. inoculated on the surface of chicken skin (Hwang & Buechat, 1995). Even though the levels of TSP used in this experiment were lower than the 10% used by Bender and Brotsky (1992), the authors found that the low levels applied for longer times were just as effective. Li et al. (1994) investigated the combined effect of low voltage, low current pulsed electrical signals and several food salts on S. typhimurium attached to chicken skins. Treatment with 1% TSP reduced Salmonella counts by 76% while the combination of electrical and TSP treatment reduced counts by 96% (1.4 logs). The bactericidal effect of a commercial blend of SAPP and orthophosphoric acid on raw poultry carcasses inoculated with NAL Salmonella typhimurium was evaluated by Rathgeber & Waldroup (1995). Addition of a 1.0 or 1.5% SAPP blend significantly reduced salmonella counts, although the researchers cautioned that the extent of reduction was related to the low pH of the rinse solution. When the pH of the rinse solution was adjusted closer to neutral, no reduction in salmonella counts was observed, although E. coli and coliform counts were significantly reduced. In addition to poultry, S. typhimurium is also a beef contaminant. Kim and Slavik (1994) inoculated fat and fascia surfaces of beef with S. typhimurium followed by rinse with 10% TSP for 15 seconds. A reduction of 0.91 and 0.51 logs was obtained on the TSP-treated fat and fascia surfaces, respectively. The greater reduction on the fat surfaces can be attributed to the removal of the fat layer by TSP and stronger entrapment of bacteria by the collagen fiber networks of the fascia surface. 5. Escherichia coli: The successful reduction in Salmonella counts by TSP on poultry surfaces led to the investigation of the effect on E.coli O157:H7. Kim and Slavik (1994) found that 1% TSP decreased E. coli counts by 1.35 and 0.92 logs on TSP-treated © 2000 by CRC Press LLC
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beef fat and fascia surfaces, respectively. 1% trisodium phosphate significantly reduced the levels of inoculated E. coli O157:H7 on alfalfa seeds, and concentrations greater than 4% precluded recovery of E. coli by direct plating, however, the bacterium was recovered by selective enrichment (Taormina & Buechat, 1999). The added heat stress (55°C) did not reduce counts further. Although TSP was effective in reducing counts without effect on seed germination, the reduction was not sufficient to justify its use since surviving cells would continue to grow during the sprouting process. Although TSP was found to be effective against surface bound E. coli in the above-mentioned studies, polyphosphates are more effective in ground meat products. Conflicting results have been obtained with different phosphate forms, with meat type and presence of spices and other additives influencing effectiveness. A commercial blend of sodium poly-, meta-, and ortho-phosphate, was ineffective on the growth and survival of E. coli O157:H7 in ground beef, and mildly effective in fresh pork sausage (Flores et al., 1996). The authors attributed these results to the lack of heat treatment to inactivate phosphatases present in meat and a possible synergistic action of the phosphate blend with the spices added to the fresh pork sausage. 6. Aeromonas hydrophila: Although 2% polyphosphate exhibited no growth inhibition of Aeromonas hydrophila, a combination of 2% polyphosphate and 3.5% NaCl completely inhibited growth in BHI media (Palumbo et al., 1995). However, this combination treatment had only a limited effect on A. hydrophila in scallops and prevented outgrowth of the organism in ground pork during refrigerated storage. 7. Fungi: Inhibition of mold growth and mycotoxin production in high-moisture corn varieties treated with various phosphates was investigated (Lebron et al., 1989). The most effective treatments were 2.0% TSPP (tetrasodium pyrophosphate), and 1 and 2% acidic sodium polyphosphate glassy (same as SHMP) added to corn in powder form. These compounds protected undamaged corn kernels against infection but also prevented infection in damaged kernels. 2% TSPP and 2% SHMP were also effective when sprayed on the corn. The treatments were effective against the inoculated mold species and also naturally occurring species. Mycotoxin production was significantly inhibited by phosphate treatment. Inhibition of Aspergillus flavus by several phosphates was observed by Knabel et al., 1991, in culture media. Addition of Mg2+ was found to reverse inhibition of A. flavus growth by TSPP, whereas addition of Mn2+ reversed the growth inhibition by SHMP. Phosphate salts have been found to be effective against powdery mildew in cucumbers (Reuveni et al., 1992a and 1993) and clusters of winegrapes (Reuveni & Reuveni, 1995), as well as northern leaf blight and common rust in maize (Reuveni et al., 1992b; 1994).
IV. SAFETY AND TOLERANCE A. Regulatory status The FDA lists nearly all food phosphates as “GRAS” (Generally Recognized As Safe). Thus, phosphates are extensively used in food products around the world, including baby formulas and health food. Food grade phosphates and phosphoric acid are approved for use by the FDA in Title 21 of the Code of Federal Regulations (CFR). In
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Parts 182 and 184, they are identified as GRAS. Under part 182, they are listed with functional groupings as follows: • Subpart B: Multiple Purpose GRAS Food Substances • Subpart F: Dietary Supplements • Subpart G: Sequestrants • Subpart I: Nutrients Applications in the Meat and Poultry industry are regulated by the USDA and are listed in Title 9 of the CFR. Specific approvals are as follows: • Part 318.7: Use in Meat Products • Part 381.147: Use in Poultry Products The USDA limits the use of phosphates in these products to 0.5% by weight of the final product. The USDA specifically prohibits the use of phosphates in fresh meat and poultry products. Meat and poultry products processed with phosphates should be labeled appropriately, and the labels must be approved by the USDA. Only clear solutions may be injected into meat and poultry. Current regulations by the FDA limit the level of phosphates in seafood to Good Manufacturing Practice (GMP) and must be labeled accordingly. Many food phosphates are also approved for use as indirect ingredients and for other applications. Specific references follow: • 21 CFR 172.892: Use in preparation of modified food starches. • 21 CFR 173.310: Use in boiler water. • 21 CFR 173.315: Use in washing or to assist in lye peeling of fruits and vegetables. • 21 CFR 175: Subpart B - For use only as components of adhesive. • 21 CFR 175: Subpart C - For use as components of cleaning. • 21 CFR 176: Indirect Food Additives – Paper and paperboard components. Since regulation of alcoholic beverages is the responsibility of the Bureau of Alcohol, Tobacco and Firearms, the approval of ammonium phosphates for treatment of wine and alcoholic juices is listed in 27 CFR 24.246. Phosphates are included in the Standards of Identity of many standardized foods, including processed cheese, processed cheese food, processed cheese spread, evaporated milk, baking powder, phosphated flour, self-rising flour, enriched self-rising flour, selfrising white corn meal, self-rising yellow corn meal, and bread, rolls and buns. B. Physiological role, RDA, and dietary intake Phosphorus is the second most abundant mineral in the body, after calcium (Sizer & Whitney, 1997). About 85% of the phosphorus occurs bound to calcium in the bones and teeth in the form of calcium phosphate (Ca3[PO4]2) and the crystal, hydroxyapatite (Ca10[PO4]6[OH] 2). The remaining phosphorus is found in extracellular fluid or inside cells. As an important component of the nucleic acids DNA and RNA, phosphorus is part of the genetic material of each cell. It occurs in cell membranes as phospholipids and plays a vital role in energy metabolism through its inclusion in high energy phosphate bonds in molecules such as ATP, and through the phosphorylation of substrates (Groff et al., 1995). Phosphorus also plays an important role as a buffering agent for cellular fluids. The 1989 U.S. RDA for phosphorus ranges from 300 to 1200 mg/day depending on age (U.S. Food and Nutrition Board, 1989). Since excess phosphorus can cause calcium
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excretion, a 1:1 or higher ratio of calcium to phosphorus in the diet is considered optimal (Feldheim, 1983). Although phosphates are used extensively as additives in food products, their estimated contribution to the total phosphorus content of the diet is varied. Based on data from the 1977 Survey of Industry on the Use of Food Additives (Committee on the GRAS List Survey-Phase III, 1979), Greger & Krystofiak (1982) estimated that food additives contributed 20-30% of the phosphorus in the diet of an average adult (assuming a daily phosphorus consumption of 1200-1700 mg). Zemel & Bidari (1983) have estimated that phosphate additives in the American diet can increase phosphorus intake by 250 to 1000 mg/day (25-100%). Although toxicity from phosphorus is rare, Yates et al. (1998) suggest a tolerable upper intake level of 4000 mg for ages 9-70 and 3000 mg for ages 70 and up. C. Nutritional effects Bell et al. (1977) determined that a high phosphate diet increased parathyroid hormone synthesis, increased urinary secretion of cyclic AMP, and contributed to bone calcium loss. Phosphate supplementation with calcium has been shown to decrease iron (Monsen et al., 1976; Steinhardt Bour, 1984) and zinc (Cabell &Earle, 1965) absorption and utilization. A detailed review of the nutritional and toxicological effects of phosphates is provided by Molins (1991).
V. SUMMARY The effects of polyphosphates on microorganisms in food products depend on various factors which influence their activity such as the category of phosphate and concentration, pH, nature of substrate, heat treatment, type and level of microbial contamination, formulation, and storage temperature (Sofos, 1989). For these reasons, food-based experiments often do not mimic the results obtained in culture media. Moreover, results from one kind of food cannot be extrapolated to other food products. Long chain alkaline polyphosphates are more effective as antimicrobial agents compared to short chain polyphosphates, although sodium acid pyrophosphate, a short chain acidic polyphosphate and TSP, an orthophosphate are very effective in certain applications. The inhibition of SAPP is related to the decrease in pH, although pH reduction by itself does not account for suppression of microbial growth. TSP, an orthophosphate, is highly effective as a surface disinfectant. For long chain polyphosphates, inhibition increases with an increase in pH. In general, higher concentrations of polyphosphates have enhanced effects. Toxin production by bacteria such as C. botulinum and S. aureus generally occurs under condition that support the growth of the bacteria, although delayed toxin synthesis has been reported under conditions which allow the bacteria to grow. The nature of the substrate, ground meat versus whole muscle, raw versus processed, affects polyphosphate activity. Hydrolysis of polyphosphates due to heating can lead to a loss in activity, thus in certain applications involving long-chain polyphosphates these compounds should be added after heat treatment. However, many foods, especially meat products, contain phosphatases, which must be inactivated by heat to maximize polyphosphate effectiveness. The presence of polyphosphates also appears to increase the sensitivity of several microorganisms to heat. Since polyphosphates function by chelating metal ions essential for microbial growth, in foods with high levels of
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cations, polyphosphates are not very effective. Interactions of polyphosphates with other polyelectrolytes such as protein, starch, and pectin must also be considered. Bacterial species differ in their sensitivity to polyphosphates. Gram-positive bacteria and mold are sensitive to polyphosphates and gram-negative bacteria are resistant to the action of polyphosphates. Level of contamination and age of the culture can also affect polyphosphate action. Synergistic effects have been reported with combinations of polyphosphates and other preservatives such as nitrites and sorbate. Sodium chloride, in some cases, enhances antimicrobial action, and in other cases, decreases effectiveness. Presence of spices may enhance activity. Certain combinations of polyphosphates and other additives such as salt have an additive effect, while other combinations elicit synergism. In the presence of other preservative agents, polyphosphates can provide added protection during storage at abuse temperatures. Polyphosphates lack the broad spectrum of activity exhibited by primary antimicrobials such as sorbate and benzoate. However, as indirect antimicrobials, polyphosphates can impart considerable protection against microbial growth and spoilage while at the same time providing physical and chemical functionality.
VI. REFERENCES 1. 2. 3. 4. 5. 6. 7.
8. 9. 10. 11. 12. 13.
14. 15. 16. 16a. 17.
Bell, R.R., Draper, H.H., Tzeng, D.Y.M., Shin, H.K., and Schmidt, G.R. 1977. Physiological responses of human adults to foods containing phosphate additives. J. Nutr. 107:42-50. Bender, F.G., and Brotsky, E. 1991. Process for treating poultry carcasses to control salmonellae growth. U.S. Patent 5,069,922. Bender, F.G., and Brotsky, E. 1992. Process for treating poultry carcasses to control salmonellae growth. U.S. Patent 5,143,739. Cabell, C.A., and Earle, I.P. 1965. Additive effect of calcium and phosphorus on utilization of dietary zinc. J. An. Sci. 24:800. Committee on the GRAS List Survey-Phase III. 1979. The 1977 Survey on the Use of Food Additives. National Academy of Sciences. Washington, D.C. Dick, W. A., and Tabatabai, M.A. 1977. Determination of orthophosphates in aqueous solutions containing organic and inorganic phosphorous compounds. J. Environ. Qual. 6:82-85. Eckner, K.F., Dustman, W.A., Rys-Rodriguez, A.A. 1994. Contribution of composition, physicochemical characteristics and polyphosphates to the microbial safety of pasteurized cheese spreads. J. Food Prot. 57:259-300. Ellinger, R.H. 1972. Phosphates as Food Ingredients. Boca Raton, FL: CRC Press. Elliott, R.P., Straka, R.P., and Garibaldi, J.A. 1964. Polyphosphate inhibition of growth of pseudomonads from poultry meat. Appl. Microbiol. 12:517- 522. Feldheim, W. 1983. On the ratio of calcium and phosphorus in human nutrition. Milchwiss. 38: 284-286. Flores, L.M., Summer, S.S., Peters, D.L., Mandigo, R. 1996. Evaluation of a phosphate to control pathogen growth in fresh and processed meat products. J. Food Prot. 59:356-359. Foster, R.D., and Mead, G.C. 1976. Effect of temperature and added polyphosphate on the survival of poultry meat during cold storage. J. Appl. Bacteriol. 41:505-510. Garibaldi, J.A., Ijichi, K., and Bayne, H.G. 1969. Effect of pH and chelating agents on the heat resistance and viability of Salmonella typhimurium TM-1 and Salmonella senftenberg 775 W in egg white. Appl. Microbiology. 18:318-322. Geise, J. 1993. Salmonella reduction process receives approval. Food Tech. 47:110. Giese, J. 1994. Antimicrobials: Assuring food safety. Food Tech. 48 : 101-110. Greger, J.L., and Krystofiak, M. 1982. Phosphorus intake of Americans. Food Tech. 36:78-84. Groff, J.L., and Gropper, S.S. 1999. Advanced Nutrition and Human Metabolism, 3rd ed. Belmont, California: Wadsworth/Thomson Learning. Hwang, C., and Beuchat, L.R. 1995. Efficacy of selected chemicals for killing pathogenic and spoilage microorganisms on chicken skin. J. Food Prot. 58:19-23.
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Jen, C. M. C., and Shelef, L.A. 1986. Factors affecting sensitivity of Staphylococcus aureus 196E to polyphosphates. Appl. Microbiol. 52: 842-846. Kim, J.W., and Slavik, M.F. 1994. Trisodium (TSP) treatment of beef surfaces to reduce Escherichia coli O157:H7 and Salmonella typhimurium. J. Food Sci. 59:20-22. Knabel, S.J., Walker, H.W., Hartman, P.A. 1991. Inhibition of Aspergillus flavus and selected gram-positive bacteria by chelation of essential metal cations by polyphosphates. J. Food Prot. 54:360-365. Kohl, W.F. 1971. A new process for pasteurizing egg whites. Food Technol. 25:1176-1184. Krzynowek, J., and Panunzio, L.J. 1995. Practical application of thin-layer chromatography for detection of polyphosphates in seafood. J. AOAC Int. 78:1328-1332. Lebron, C.I., Molins, R.A., Walker, H.W., Kraft, A.A., and Stahr, H.M. 1989. Inhibition of mold growth and mycotoxin production in high- moisture corn treated with phosphates. J. Food Prot. 52:329-336. Lee, R.M., Hartman, P.A., Olson, D.G., Williams, F.D. 1994a. Bacterial and bacteriolytic effects of selected food-grade phosphates using Staphylococcus aureus as a model system. J. Food Prot. 57:276-283. Lee, R.M., Hartman, P.A., Olson, D.G., Williams, F.D. 1994b. Metal ions reverse the inhibitory effects of selected food-grade phosphates in Staphylococcus aureus. J. Food Prot. 57:284-288, 300. Lee, R.M., Hartman, P.A., Stahr, H.M., Olson, D.G., Williams, F.D. 1994c. Antibacterial mechanism of long-chain polyphosphates in Staphylococcus aureus. J. Food Prot. 57:289-294. Li, Y., Kim, J-.W., Slavik, M.F., Griffis, C.L., Walker, J.T., and Wang, H. 1994. Salmonella typhimurium attached to chicken skin reduced using electrical stimulation and inorganic salts. J. Food Sci. 59:23-29. Loessner, M.J, Maier, S.K., Schiwek, P., and Scherer, S. 1997. Long-chain polyphosphates inhibit growth of Clostridium tyrobutyricum in processed cheese spreads. J. Food Prot. 60:493-498. Matsuoka, A., Tsutsumi, M., Watanabe, T. 1995. Inhibitory effect of hexametaphosphate on growth of Staphylococcus aureus. J. Food Hyg. Soc. Japan. 36:588-594. Molins, R.A. 1991. Phosphates in Foods. Boca Raton, FL: CRC Press. Molins, R.A., Kraft, A.A., and Marcy, J.A. 1987. Extension of the shelf-life of fresh ground pork with phosphates. J. Food Sci. 52:513-514. Molins, R.A., Kraft, A.A, Olson, D.G., and Hotchkiss, D.K. 1984. Recovery of selected bacteria in media containing 0.5% food grade poly- and pyrophosphates. J. Food Sci. 49:948-949. Monsen, E.R. and Cook, J.D. 1976. Food iron absorption in human subjects. IV. The effects of calcium and phosphate salts on the absorption of nonheme iron. J. Clin. Nutr. 29:1142-1148. Murphy, J., and Riley, J.P. 1962. A modified single solution method for the determination of phosphate in natural waters. Anal. Chim. Acta. 27:13-36. Palumbo, S.A., Call, J.E., Cooke, P.H., Williams, A.C. 1995. Effect of polyphosphates and NaCl on Aeromonas hydrophila K144. J. Food Safety. 15:77-87. Post, F.J., Colbentz, W.S., Chou, T.W., and Salunkhe, D.K. 1968. Influence of phosphate compounds on certain fungi and their preservative effect on fresh cherry fruit. Appl. Microbiol. 16:138-142. Prasad, S., and Prasad, C. 1989. Phosphates in dairy and food industries. Indian Dairyman 41:121- 126. Rajkowski, K.T, Calderone, S.M., and Jones, E. 1994. Effect on polyphosphate and sodium chloride on the growth of Listeria monocytogenes and Staphylococcus aureus in ultra- high temperature milk. J. Dairy Sci. 77:1503-1508. Rathgeber, B.M., and Waldroup, A.L. 1995. Antibacterial activity of sodium acid pyrophosphate product in chiller water against selected bacteria on broiler carcasses. J. Food Prot. 58:530-534. Reuveni, M., Agapov, V., and Reuveni, R. 1992a. Local and systemic resistance against powdery mildew and growth increase in cucumber plants induced by phosphate salts. (Abstr.) Phytopath. 82:1179. Reuveni, M., Agapov, V., and Reuveni, R. 1992b. Systemic resistance against northern leaf blight and common rust in maize induced by foliar spray of phosphates. (Abstr.) Phytopath. 82:1179. Reuveni, M., Agapov, V., and Reuveni, R. 1993. Induction of systemic resistance to powdery mildew and growth increase in cucumber by phosphates. Biol. Agric. Hort. 9:305-315. Reuveni, M., Agapov, V., and Reuveni, R. 1994. Foliar spray of phosphates induces growth increase and systemic resistance to Puccinia sorghi in maize. Plant Path. 43:245-250. Reuveni, M., and Reuveni, R. 1995. Efficacy of foliar application of phosphates in controlling powdery mildew fungus on field-grown wine grapes: effects on cluster yield and peroxidase activity in berries. J. Phytopath. 143:21-25. Seward, R.A., Deibel, R.H., and Lindsay, R.C. 1982. Effects of potassium sorbate and other antibotulinal agents on germination and outgrowth of Clostridum botulinum type E spores in microcultures. Appl. Environ. Microbiol. 44:1212-1221.
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Shelef, L.A., and Seiter, J.A. 1993. Indirect antimicrobials. In Antimicrobials in Foods, eds. P.M. Davidson and A.L. Branen, pp. 539-570. New York: Marcel Dekker, Inc. Shelef, L.A., and Wang, Z.L. 1989. Effects of polyphosphates on cell numbers, enterotoxins A, and extracelluar protein in Staphylococcus aureus 196E. J. Food Sci. 54:1550-1552. Shelef, L.A, Wang, Z.L., and Udeogu, A.C. 1990. Growth of Staphylococcus aureus and enterotoxin A production in foods containing polyphosphates. J. Food Safety. 10:201-208. Sizer, F.S., and Whitney, E.N. 1997. Nutrition: Concepts and Controversies, 7th ed. California: Wadsworth Publishing Company. Sofos, J.N. 1989. Phosphates in meat products. In Developments in Foods Preservation, ed. S. Thorne, pp.207-252 . Barking, U.K: Elsevier. Steinhardt Bour, N.J., Soullier, B.A., and Zemel, M.B. 1984. Effect of level and form of phosphorus and level of calcium intake on zinc, iron and copper bioavailability in man. Nutr. Res. 4:371. Taormina, P.J., Beuchat, L.R. 1999. Comparison of chemical treatments to eliminate enterohemorrhagic Escherichia coli O157: H7 on alfalfa seeds. J. Food Prot. 62:318-324. Tarr, H.L.A., Gardner, L.J., and Ingram, P. 1969. Pacific cod muscle 5’ nucleotidase. J. Food Sci. 34: 637-640. Tompkin, R.B. 1984. Indirect antimicrobial effects on foods: Phosphates. J. Food Safety. 6:13-27. Tsuji, S., Shibata, T., Uchibori, N., Kobayashi, T., Suzuki, H., Uchibori H.S., Muroi, J., Kaneda, N., and Ito, Y. 1994. J. Food Hyg. Soc. Jap. 35(1): 56-65. U.S. Food and Nutrition Board. 1989. Recommended Dietary Allowances, 10th ed., National Academy of Sciences, National Research Council, Washington, D.C. Van Wazer, J.R. 1971. Chemistry of phosphates and condensed phosphates. In Symposium: Phosphates in Food Processing, eds. J.M. Deman, and P. Melnychyn, chap. 1, Westport, CN: AVI Publishing. Van Wazer, J.R., and Callis, C.F. 1958. Metal complexing by phosphates. Chem. Rev. 58:1011-1046. Vishniac, W. 1950. The antagonism of sodium tripolyphosphate and adenosine tryphosphate in yeast. Arch. Biochem. 26:167-172. Wagner, M.K. 1986. Phosphates as antibotulinal agents in cured meats: A review. J. Food Prot. 49:482487. Wagner, M.K., and Busta, F.F. 1985. Inhibition of Clostridium botulinum 52A toxicity and protease activity by sodium acid pyrophosphate in media systems. Appl. Environ. Micribiol. 50:16-20. Wood, H.G., and Clark, J.E. 1988. Biological aspects of inorganic polyphosphates. Ann. Rev. Biochem. 57:235-260. Yasuno, T., Funayama, K., Hagiwara, T., and Suzuki, S. 1996. Determination of orthophosphates in condensed phosphates used as food additives by ion chromatography. Ann. Rep. Tokyo Metro. Res. Lab. Pub. Health. 47:189-193. Yates, A., Schlicker, S., and Suitor, C. 1998. Dietary reference intakes: the new basis for recommendations for calcium and related nutrients, B vitamins and choline. J. Am. Diet. Assoc. 98:699-706. Zaika, L.L., and Kim, A.H. 1993. Effect of sodium polyphosphates on growth of Listeria monocytogenes. J. Food Prot. 56:577-580. Zaika, L.L, Scullen, O.J, and Fanelli, J.S. 1997. Growth inhibition of Listeria monocytogenes by sodium polyphosphate as affected by polyvalent metal ions. J. Food Sci. 62:867-896, 872. Zemel, M.E. and Bidari, M.T. 1983. Zinc, iron, and copper availability as affected by orthophosphates, polyphosphates and calcium. J. Food Sci. 48:567-573.
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I. INTRODUCTION Chlorine, a member of the halogen family, serves as a building block for several synthetic molecules that exhibit potent antimicrobial properties. These molecules range from simple elemental forms of diatomic chlorine, to complex organic chloramines. In this chapter, these molecules are referred to as ‘chloro-cides’. Among the various chloro-cides available today, elemental chlorine was the first to be discovered (Baldwin, 1927). At ambient conditions, elemental chlorine exists as a greenish-yellow gas with a penetrating odor. In 1774, Swedish chemist Karl W. Scheele obtained the gas by oxidizing nascent HCl with MnO2. Scheele observed that the gas was soluble in water, and demonstrated a permanent bleaching effect on paper, vegetables, and flowers. These properties brought chlorine to its first commercial use, as bleaching agent for the textile industry. Later in 1789, in a French chemical plant in Javel, Berthollet improved the bleaching action of chlorine solution by mixing it with potassium hydroxide. The resulting compound was a hypochlorite (OCl-) solution termed ‘Javelle water’ after the name of the town where it was discovered. Later, Labarraque modified the manufacturing process of hypochlorite by replacing potassium hydroxide with inexpensive sodium hydroxide, commonly known as caustic soda. Chlorination of sodium hydroxide remains the most popular method for the production of hypochlorite. Shortly after the discovery of sodium hypochlorite, the discovery of lithium- and calcium-hypochlorites followed. Later, various antimicrobial properties of hypochlorite were discovered. In 1881, a German bacteriologist, Robert Koch, demonstrated the activity of hypochlorites to destroy pure cultures of bacteria under controlled laboratory conditions. By end of the nineteenth century, the American Public Health Association (APHA) recognized hypochlorites as potent broad-spectrum antimicrobial agents (Hadfield, 1957). The first commercial use of chlorine compound for disinfection was in the form of hypochlorite. It was used in London during 1850 to treat a contaminated water supply that had led to an outbreak of cholera.
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Natural Food Antimicrobial Systems
Since the discovery of chlorine and hypochlorites, many other chlorine compounds were discovered that had distinct advantages as antimicrobial agents. A variety of organic chloro-cides were discovered that were not as susceptible to photo-decomposition as elemental chlorine or hypochlorite. They provided better disinfection properties for treating exposed water environments such as swimming pools, ponds, and open reservoirs. The organic chlorinating agents were also helpful in reducing metal corrosion on equipment used in the processing of water or food. Moreover, these compounds released hypochlorous acid in a sustained manner, preventing the liberation of chlorine gas. Many organic chloro-cides were also used in medical applications. Dakin et al. (1916) used Chloromine-T during World War I for treating infected wounds. Thereafter, Leech (1923) reported the germicidal properties of various organic chloro-cides. The discovery of chlorine dioxide (ClO2) was reported by Humphry Davy, soon after he declared chlorine to be an element. The antimicrobial effectiveness of ClO2 was soon elucidated. However, due to its energetic nature, the use of ClO2 did not become widespread. Greater than 15% concentration of ClO2 in confined spaces is a potential explosive. Therefore, compressed ClO2 could not be packaged into cylinders for shipping. It must be produced at the site of application. The first on-site generation of ClO2 was reported in 1944, when it was used for the disinfection of water at the Niagara Falls (Aston, 1947). Since then, the generation technology for ClO2 has undergone major breakthroughs and currently it is widely used for disinfection and sanitation in various applications. In recent times, the use of certain chlorine compounds has faced opposition from environmentalists. A number of studies indicated that chlorine-based compounds form carcinogenic by-products (Richardson et al. 1998). A chloro-cide that is exempted from these controversial issues is ClO2. The oxidation mechanism of ClO2 is fundamentally different than other chlorine based compounds and therefore, it does not produce any detectable levels of chlorinated organic by-products. Due to the continued pressure to control disinfection by-products (DBP) by the Environmental Protection Agency (EPA), ClO2 has received a great deal of attention. The focus on ClO2 is increasing due to its potent sanitizing efficacy and for not forming any carcinogenic by-products. Therefore, this chapter will discuss the molecular mechanisms of ClO2 more in detail than the other chloro-cides.
II. STRUCTURE AND CHEMISTRY Natural forms of chlorine display only a single oxidation state where it exists as a monovalent chloride anion in the form of carnallite (KMgCl3, 6H2O), sylvite (KCl) and common salt (NaCl). None of the natural forms have any unique antimicrobial properties. The synthetic compounds of chlorine, however, could demonstrate oxidation states ranging from -1 to +7 (Taube et al., 1949). Such a wide range of possible oxidation states of chlorine results in a plethora of chloro-cides that satisfy the diverse needs of the sanitation and disinfection industry. A list of these compounds and their structures are listed in TABLE 1 and FIGURE 1. Further details regarding the commercially important compounds are discussed under four subsections: elemental chlorine, inorganic chloro-cides, organic chloro-cides and chlorine dioxide. ClO2 being an inorganic chloro-cide is elaborated under a separate header, as it is considered different from most chlorinating agent in terms of activity and residual byproducts. © 2000 by CRC Press LLC
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TABLE 1. Antimicrobial chloro-cides commonly used in the industry Chemical Name [CAS No.]
Formula
Inorganic compounds Chloramines Sodium hypochlorite [7681-52-9] Calcium hypochlorite [7778-54-3] Lithium hypochlorite [13840-33-0] Chlorinated trisodium phosphate [56802-99-4] Chlorine dioxide [10049-04-4]
NHxCly NaOCl Ca(OCl)2 LiOCl 4(Na2PO4.11H2O)NaOCl ClO2
Organic compounds Sodium benzenesulfonchloramide [127-52-6] (Chloramine-B) Sodium p-toluene sulfonchloramide [127-65-1] (Chloramine-T) p-Toluene sulfonchloramide [473-34-7] (Dichloramine-T) p-Sulfondichloramidobenzoic acid [80-13-7] (Halazone) Trichloroisocyanuric acid [87-90-1] (Symclosene) Sodium dichloroisocyanurate [51580-86-0] Potassium dichloroisocyanurate [2244-21-5] Trichloromelamine [7673-09-8] 1,3-Dichloro-5,5-dimethyl hydantoin [118-52-5] (Halane) N-Chlorosuccinimide [128-09-6] N,N”-dichlorodiazenedicaboximidamide [502-98-7] (Chloroazodin)
C6H4ClNNaO2S p-CH3C6H4SO2NClNa p-CH3C6H4Cl2NO2S p-C7H5Cl2NO4S C3Cl2N3O3 Na[C3Cl2N3O3] K[C3Cl2N3O3] C3H3Cl2N6 C5H6Cl2N2O2 C4H4ClNO2 C2H4Cl2N2
The availability of several different chloro-cides is often overwhelming to an end user. In general, a user considers replacement of one sanitizer with another for reasons related to efficacy, convenience, or cost. In such a case, it is useful to compare the biocidal efficiencies of chloro-cides by calculating their ‘available chlorine’ content. Available chlorine is a measure of the oxidizing capacity of a compound as compared to elemental chlorine. It is calculated by determining the electrochemical equivalent amount of Cl2 to that compound. Available chorine content provides a normalized scale for comparing the efficiencies of various sanitizers. For example, compare NaOCl with Ca(OCl)2. It could be deduced from Equation 1 and Equation 2 that the electrochemical reactions of elemental chlorine and the hypochlorite ion, each proceed with a consumption of two electrons. Therefore, it may be concluded that electrochemically, one mole of elemental chlorine is equivalent to one mole of hypochlorite. Since the molecular weight of Cl2 is 70.91 g, one mole of hypochlorite shall contain 70.91 g of available chlorine. Accordingly, one mole of NaOCl contains 70.91 g of available chlorine, whereas, one mole of Ca(OCl)2 contains 141.8 g of available chlorine. Cl2 + 2e- ← 2Cl-
-
OCl + 2e + 2H
+
(Equation 1)
← Cl + H2O -
(Equation 2)
Although the ‘available chlorine’ scale provides a good general tool for comparing the biocidal efficacy of chloro-cides, one must be cautious in using this concept when ClO2 is compared with another chloro-cide. According to Equation 3, the electrochemical reaction of ClO2 consumes 5 electrons which is 2.5 times more than that of elemental chlorine. Therefore, the available chlorine content in one mole of ClO2 is 177.3 g (obtained from 70.91 x 2.5). Since the molecular weight of one mole of ClO2 is 67.45, it is expected to be 2.63 times more potent than elemental chlorine (2.63 is obtained from
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FIGURE 1. Structures of commercially produced organic chloro-cide compounds.
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177.3/67.45). However, it has been observed that the biocidal efficacy of ClO2 is greater than two orders of magnitude when compared to that of chlorine (Tanner, 1989). This may be due to the difference in the mechanism of the two biocides. ClO2 + 5e- + 4H+
← Cl- + 2H2O
(Equation 3)
A. Elemental chlorine Elemental chlorine is a widely used disinfectant (White, 1992). Although at ambient conditions it exists as a gas, it can be safely compressed into a liquid form. Liquid chlorine is easier to handle and cheaper to transport. The first liquification process of chlorine was demonstrated in 1805 by Thomas Northemore by compressing the gas into a clear amber-colored liquid. It was noted that upon release of pressure, the liquid rapidly volatilized into gaseous form. The gaseous form of chlorine is yellowish-green in color. Green translates as ‘chloros’ in Greek, and is the root of the name ‘chlorine’ as nomenclatured by Humphry Davy. He also declared chlorine to be an element in 1811 after unsuccessful attempts to effect its decomposition. Elemental chlorine proves economical in high volume uses such as in the treatment of water and wastewater. A substantial amount of chlorine is used in the power industry to prevent biofouling of heat exchangers. For majority of antimicrobial applications, chlorine is converted into other chlorine compounds such as hypochlorites, which provide ease of use and safe handling. On a commercial scale, chlorine is manufactured by electrolysis of brine with an overall reaction according to Equation 4. NaCl + H2O + electric current
← NaOH + 1/2 Cl2 + 1/2 H2
(Equation 4)
Differences in the manufacturing processes of chlorine are primarily based in the types of electrolytic cells used, i.e. diaphragm, mercury and membrane (White, 1992). In 1998, about 12.8 million tons of chlorine was produced in the United States (C&E News, 1999). An estimated one million tons have been used in the treatment of drinking water and wastewater. In aqueous solutions, chlorine disproportionates according to Equation 5. Cl2 + H2O ← HOCl + H+ + Cl-
(Equation 5)
The major pathway for the above reaction is via hydroxyl ion where the rate approaches to that of the diffusion control reactions (Morris, 1692). This is of great practical significance since the rapid kinetics of this reaction enable high passage of aqueous chlorine solutions from chlorine generators without degassing problems. The properties of gas and liquid phase chlorine are listed in TABLE 2. B. Inorganic chloro-cides The two primary chlorine compounds that fall under this category are hypochlorites and chloramines. 1. Hypochlorites. Hypochlorites are the oldest and the most widely used antimicrobial agents for sanitation and disinfection. They are commonly known as bleach and their biggest application is in the treatment of potable water and wastewater. Although the
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TABLE 2. Properties of chlorine Symbol Molecular weight Solubility in water (68˚F) Molar absorptivity in water (325 nm) Gas: Density (34˚F) Viscosity (68˚F) Liquefying point Liquid: Boiling point Freezing point Density (32˚F) Viscosity (68˚F) 1 volume liquid at 32˚F,1 atm 1 kg liquid at 32˚F, 1 atm
Cl2 70.914 g/mol 7.29 g/L 75 cm-1 M-1 0.00321 g/ml 0.01325 centipoise -30.1˚F (-34.5˚C) -30.1˚F (-34.5˚C) -149.8˚F (-101.0˚C) 1.47 g/ml 0.345 centipose 457.6 vol gas 310.2 L gas
cost of hypochlorites is approximately two to four times higher than that of chlorine gas, use of the former is growing due to the risk of chlorine accidents. This is particularly true in large metropolitan areas where high volume of disinfectant is required for water treatment. The hypochlorite ion is comprised of chlorine and an oxygen molecule with an overall negative charge, ClO-. The common counter cations of OCl- that are used in the industry are Na+, Li+ and Ca2+. Sodium hypochlorite (NaOCl), also known as soda bleach liquor or liquid bleach, is the most widely used of all the chlorinated bleaches. In the United States, more than 150 tons of sodium chlorite is used every day (White, 1992). The use of sodium hypochlorite is preferred over other hypochlorites due to its low cost and ease of handling. Sodium hypochlorite has the least maintenance problems with pumping and metering equipment. Moreover, there is no fire hazard associated with its storage. Sodium hypochlorite is often supplied as a mixture with trisodium phosphate (TSP). This product is known as chlorinated TSP. Chlorinated TSP provides the benefits of disinfection along with the cleaning action of TSP. Sodium hypochlorite is manufactured by reacting gaseous chlorine with the solution of caustic soda as shown in Equation 6. Cl2 + NaOH
← NaOCl + NaCl + H2O + Heat
(Equation 6)
To improve the stability of the product, more caustic soda is added than suggested by the reaction stoichiometry. The commercially available solutions of sodium hypochlorite are as high as 15% available chlorine in concentration. More concentrated solutions cause purification problems due to solidification. Calcium hypochlorite solutions are made by passing chlorine into milk of lime suspension according to Equation 7. 2Cl2 + 2Ca(OH)2
← Ca(OCl)2 + CaCl2 + 2 H2O
(Equation 7)
The maximum strength of these solutions is limited to about 35% available chlorine. These solutions are prone to sludge formation caused by the presence of impurities such as magnesium or aluminum oxides. Therefore, calcium hypochlorite is not desired in
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operations where sophisticated metering equipment is involved. The potential insolubles result in maintenance problems. Due to the much higher available chlorine content of calcium hypochlorite, it is used in remote areas where the transportation cost becomes significant. Calcium hypochlorite is also commercially available in granular form where the available chlorine content is 65 to 70%. Granular calcium hypochlorite is the most common form of dry bleach used in the industry. Granular calcium hypochlorite in concentrations greater than 35% is a fire hazard and must be stored away from heat and oxidizable organic compounds. Although manufacturers use different approaches for the production of granulated calcium hypochlorite, the basic process involves chlorination of lime slurry. Among the granulated forms of hypochlorites, lithium hypochlorite is another prevalent form. It is prepared by mixing strong solutions of lithium chlorite and sodium hypochlorite, followed by evaporation of the reaction mixture. Lithium hypochlorite is a clean and free-flowing form of granulated hypochlorite, which is readily soluble in water. Therefore, it has distinct advantages over calcium hypochlorite such as that the solution 1) does not contain any sludge, 2) does not significantly affect the alkalinity or the pH of water and 3) is relatively more stable in the solution form. Degradation of active components during storage is a major problem with hypochlorite solutions (Gordon, 1997). The loss is proportional to the exposure to light and heat. The presence of heavy metal cations such as iron, copper, nickel, and cobalt, adversely affect the stability of hypochlorite solutions. For maximum shelf life of hypochlorite solutions, dilution to a low concentration (~10%) is recommended. The presence of heavy metal ions should be minimized (preferably 9.0. Hypochlorites are sold at alkaline pH and are to be mixed with acids for effective sanitation. Lowering of pH facilitates hydrolysis that produces the primary biocidal component, HOCl. The addition of acids in the hypochlorite systems must be performed with caution since at low pH they start liberating hazardous chlorine gas. Depending on the type application, the chlorinating systems are typically operated between the pH of 6.5 and 7.5. The role of pH in antimicrobial efficacy of chlorine is well documented (Dychdala, 1983). The pH also plays a critical role in the sporicidal efficacy of hypochlorite. Most commercial hypochlorite solutions produce a slightly alkaline pH at their use dilution. The antimicrobial properties of chlorine are not favorable under alkaline conditions. As compared to various chlorinating systems, the pH range of ClO2 is more flexible. ClO2 does not ionize in water, and therefore its bactericidal efficiency remains essentially constant over the normal range of pH values in natural water (Ridenour & Ingols, 1947; Bernarde et al., 1965). Owing to its high solubility, the release of gas from the solution at low pH is much less as compare to chlorine. Once generated and introduced into the use solution, ClO2 is effective up to pH 10.0. At pH values >10.0, ClO2 slowly starts converting into ClO2-. Bernarde et al. (1965) found that equivalent concentrations of ClO2 and hypochlorite at pH 8.5 produced an equivalent degree of cidal activity against E. coli in 15 and 300 s, respectively. At pH 6.5, the two compounds were almost equally effective at equivalent concentrations.
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Berman et al. (1984) studied the effect of chlorine, ClO2, and monochloramine on viruses at 5˚C at pH 6 and 10. The results indicated that 0.5 ppm (as Chlorox), inactivated virions in less than 15-s at pH 6.0, resulting in 4-log reduction, but not at pH 10. With chlorine dioxide, however, 0.5 ppm was more efficient at pH 10 than at pH 6.0, with a 15-s inactivation. Monochloramine at 10 ppm concentration and pH 8.0 required more than 6 h to produce an equivalent inactivation of virions. 3. Temperature: The destruction of microorganisms follows first order kinetics. According to the Arrhenius relationship the reaction rate (biocidal activity) doubles with every 10˚C (18˚F) change in temperature (Wilkins, 1991). However, higher temperatures adversely affect the solubility, and gassing-off becomes a concern. The effects of temperature on the antimicrobial activity of chlorine is well documented (Trueman, 1971; Dychdala, 1983). At high concentrations of chlorine, the temperature effect is not readily apparent; however, at low concentrations the effect is multifold. Johns (1954) found no difference in the rate of kill for hypochlorite against Micrococcus pyogenes var. aureus, E. coli, or Pseudomonas aeruginosa at approximately 10 ppm and temperatures of 5, 20, and 40˚C. These results also indicate that although hypochlorite is sensitive to temperature effects, it is significantly less sensitive than the other commonly used sanitizers. Rudolph and Levine (1941) found a pronounced temperature effect on the spores of B. metiens. Temperature sensitivity data for the organic chlorine compounds are not readily available. Johns (1954) found that a dichlorodimethylhydantoin product was more temperature sensitive than hypochlorites, especially for P. aeruginosa. Decrease in temperature from 45 to 5˚C necessitated a 4-fold increase in organic chlorine content to achieve the same rate of kill. Bernarde et al. (1967a) evaluated the effect of temperature on ClO2 disinfection. A substantial temperature effect was observed over the temperature range of 5-32˚C; however, no direct comparison to temperature effects on hypochlorite was established. Ridenour and Ingols (1947) showed a lower antimicrobial activity for ClO2 at lower temperature and demonstrated that pH in range of 6-10 had no special effect on its activity. 4. Organic load: Organic matter in the milieu significantly affect the bactericidal efficacy of chlorine compounds (Trueman, 1971; Dychdala, 1983). Johns (1954) studied the activity of various sanitizing solutions in the presence of 0.5% skim milk at varying temperatures. The organo-chlorine compound dichlorodimethylhydantoin was less sensitive to the addition of organic material than hypochlorite solution. Bloomfield and Miles (1979b) compared the antimicrobial effect of sodium hypochlorite and sodium dichloroisocyanurate in the presence of organic material. Both chlorine compounds demonstrated equivalent cidal activity in the absence of organic material, however, an abrupt change in the antimicrobial efficacy was observed as the milk concentration increased from 0.5 to 2.0%. ClO2 is a highly reactive compound, but as chlorine, it does not react with ammonia and other nitrogenous compounds and in general, is not as susceptible to the effects of organic matter (White, 1972). Lillard (1979) found that ClO2 was significantly more effective than chlorine in reducing the aerobic and fecal coliform counts in poultry processing water.
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5. Water quality: Alkalinity, hardness and organic load content of water affect the efficacy of a sanitizer. The effect of alkalinity could be seen particularly in cases where sanitizers are used for stasis of microorganisms. The mechanism of stasis involves reaction of acidic metabolites of the organism with the biocide precursor. High alkalinity (CO32- and HCO3- ions) neutralize the acid produced by microorganism preventing the production of the active ingredient. With extremely hard water (>500 ppm), the hypochlorites form precipitates. Water hardness per se does not exert a marked effect on the antimicrobial activity of chlorine. However, in many cases, hard water could cause an upward drift in pH and diminish chlorine efficacy (Hays et al., 1967; Mosley et al., 1979) 6. Mode of application: The sanitizer could be applied by various delivery mechanisms including circulating, submerging, brushing, fogging, or spraying systems. Automation of the beverage industry has led to the increased use of clean-in-place (CIP) systems managed by computer-controlled valves and pumps. Sanitation of these systems entails circulating sanitizer through pipelines. For effective sanitation of tanks and vats, scrubbing is required to detach food particles and biofilm. Fogging is an effective way to reduce microorganisms from air that are potential risk for product contamination. Jeng and Woodworth (1990) studied ClO2 gas sterilization under square-wave conditions. By using controlled humidity, gas concentration, and temperature at atmospheric pressure, standard biological indicators and spore disks of environmental isolates were exposed to ClO2 gas. Prehumidification enhanced the ClO2 activity. The D values (time required for 90% inactivation) of Bacillus subtilis ssp.niger were estimated to be 1.5, 2.5 and 4.2 min when exposed to ClO2 concentration of 30, 15, and 7 mg/L, respectively, at 23˚C and ambient (20-40%) relative humidity (FIGURE 2). The study indicated that ClO2 gas on a molar basis was 1,075 times more potent than ethylene dioxide as a sterilant at 30˚C. C. Microbial resistance Vegetative bacteria are generally more susceptible to chlorine inactivation than microorganisms that form spores. Based on free available chlorine concentration and contact time, bacterial spores are 10-10,000 times more resistant to destruction by chlorine than vegetative cells (Ito & Seeger, 1980; Odlaug, 1981). Several authors (Johns, 1934, 1948; Trueman, 1971; Mosely et al., 1976) have observed a greater resistance in certain strains of Staphylococcus aureus compared to pseudomonads and other Gram-negative bacteria. With other commonly used sanitizers and disinfectants, notably quaternary ammonium compounds, the reverse is generally true. Haas and Engelbrecht (1980) suggested that yeasts and acid-fast bacteria would be more appropriate indicators of water disinfection than E. coli because of their greater resistance to free available chlorine. A comprehensive report published by the EPA (1979) ranked Mycobacterium fortuitum and Candida parapsilosis well ahead of E. coli in resistance to chlorine. Bolton (1988) showed that strains of S. aureus isolated from biofilms and collected from the defeathering equipment were almost 8-fold more resistant than strains from the natural skin flora of poultry. It was concluded that the resistance of these strains was due to their ability to form macroclumps by production of an extracellular slime. Caldwell (1990) reported that low chlorine levels (0.5-5 ppm) are only inhibitory to biofilms and their cells. Higher chlorine level of 50 ppm and up was needed for the reduction of biofilms by biocidal action. El-Kest and Marth (1988) tested L. monocto© 2000 by CRC Press LLC
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genes against sodium hypochlorite and concluded that a good program of cleaning and sanitizing should be able to control non-spore-forming organisms, including L. monocytogenes. Acquired resistance to chlorine has not been demonstrated; however, Scheusner et al. (1971) provided evidence for chlorine-induced sublethal injury in E. coli by exposure to 1 µg/ml of hypochlorite. Stress resulting from a variety of chemical and physical environments has been recognized in indicator bacteria. Indicator microorganisms are sublethally impaired due to a variety of causes associated with foods. Workers in the area of water microbiology are also gaining an appreciation of the importance of these stressed cells in the assessment of water quality using bacterial indicators. Chemical agents, including chlorine, which are employed in water disinfection processes, are important causes of bacterial stress injury. Ojajarvi and Makela (1976) studied the disinfecting properties of chloramine and compounds containing chlorinated trisodium phosphate and potassium bromide or sodium dichloroisocyanurate and detergents. They found that the effectiveness of chlorinebromine disinfectant substantially decreased in the presence of organic material. Irritation of the skin and the mucus membranes when using chlorine disinfectants was also observed. Bacteria located within microbial aggregates (formed by flocculation during water treatment) are protected against chlorine. Enterobacter cloacae attached to drinking water distribution particles are also protected from chlorine disinfection. This effect was dependent on the level of chlorine in the system and attachment time (Herson et al., 1987). Indigenous coliforms associated with the particle fractions were tested for resistance to chlorine and monochloramine (Berman et al., 1988). Coliforms associated with < 7-µ fraction were inactivated more rapidly by 0.5 mg of chlorine per liter at 5˚C and pH 7 than coliforms associated with > 7-µ fraction. The time required for 99% inactivation of the particle fractions with monochloramine at pH 7 or 8 was 20- to 50-fold greater than the time required for the same amount of inactivation with chlorine at pH 7. These results indicate that coliforms associated with sewage effluent particles are inactivated more rapidly with 0.5 mg of chlorine per liter than with 1.0 mg of monochloramine per liter. However, > 7-µ particles have a protective effect against the disinfecting action of chlorine. Lisle and co-workers (1998) reported that chlorine resistance in E. coli O157:H7 progressively increased through the starvation period. After 29 days of starvation, there was no significant difference in chlorine resistance between control cultures that had not been exposed to the disinfectant and cultures that had been exposed. This study suggested that E. coli O157:H7 adapts to starvation conditions by developing a chlorine resistance phenotype. D. Storage stability The stability of sodium hypochlorite (diluted household bleach) when stored for 30 days in various types of containers and the efficacy of low concentrations of free available chlorine to inactivate bacteria was tested (Rutala et al., 1998). Solutions of standard household bleach were prepared using tap water or sterile distilled water at dilutions of 1:100, 1:50, and 1:5. Chlorine concentrations were measured, and the solutions were left in polyethylene containers at room temperature (20˚C) under various conditions (translu-
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cent containers with light exposure and with or without air; brown opaque container without light or air exposure). Samples for chlorine and pH determinations were taken at time 0 and on days 7, 14, 21, 30, and 40. Bactericidal activity of chlorine solutions was assessed against strains of Pseudomonas aeruginosa, Staphylococcus aureus, and Salmonella choleraesuis. Chlorine concentrations at 30 days varied from the 40% to 50% range for 1:50 or 1:100 dilutions stored in containers other than closed brown containers to 83% to 85% for the 1:5 dilution stored in closed but non-opaque containers to 97% to 100% for 1:50 or 1:5 solutions stored in closed brown containers. The lowest concentration of sodium hypochlorite solution that reliably inactivated all the test organisms was 100 ppm. These data suggest that chlorine solutions do not need to be prepared fresh daily and 100 ppm concentration of chlorine effectively inactivates S. aureus, S. choleraesuis, and P. aeruginosa.
IV. ANTIMICROBIAL SPECTRUM Chloro-cides can be considered a broad-spectrum germicide. Hypochlorites have documented antimicrobial activity against viruses, non-acid-fast bacteria, acid-fast bacilli, bacterial spores, fungi, algae, and protozoa (Dychdala, 1983a). The antimicrobial spectrum of chlorine is shown in TABLE 4. A. Antibacterial activity Many Legionella infections are acquired through inhalation or aspiration of drinking water and about 25% of municipalities in the USA use monochloramine for disinfection of drinking water. In a case study, Kool and coworkers (1999) concluded that 90% of outbreaks of Legionnaires’ disease associated with drinking water might not have occurred if monochloramine had been used instead of free chlorine for residual disinfection. The authors suggested that chloramination of drinking water may be a cost-effective method for control of Legionnaires’ disease at the municipal level or in individual hospitals, and widespread implementation could prevent thousands of cases. However, Legionellae are more resistant to chlorine than coliforms (Kuchta et al., 1983). At 21˚C, pH 7.6, and 0.1 mg of free chlorine residual per liter, a 99% kill of Legionella pneumophila was achieved within 40 min, compared with less than 1 min for E. coli. The observed resistance is enhanced as conditions for disinfection become less optimal. The required contact time for the removal of L. pneumophilia was twice as long at 4˚C than it was at 21˚C. These data suggest that legionellae can survive low levels of chlorine for relatively long periods of time. Lopes (1986) reported that 100 ppm available chlorine as sodium hypochlorite and dichloroisocyanurate was effective for the 5-log reduction of L. monocytogenes and Salmonella typhimurium within 30-s. The susceptibility of a strain of Legionella pneumophila to disinfection by an organic halamine, free chlorine, and a mixture of organic halamine and free chlorine was reported (Swango et al., 1987). The organic halamine had superior stability in solution and exhibited adequate disinfectant potential over a period of 1 month of repeated reinoculations of fresh bacteria. The combined halamine exhibited great potential for use in maintaining closed-cycle cooling water systems free of L. pneumophila. Water disinfection systems utilizing electrolytically generated copper and silver ions (200 and 20, 400 and 40, or 800 and 80 µg/L) and low levels of free chlorine (0.1 to 0.4 mg/L) were evaluated at room (21 to 23˚C) and
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TABLE 4. Antimicrobial spectrum of chlorine. Bacterial species Antibacterial activity Aerobacter aerogenes Aeromonas hydrophila / A. caviae Alcaligenes faecalis Bacillus cereus/ B. cereus Bacillus macerans Bacillus stearothermophilus Bacillus coagulans Campylobacter jejuni Clostridium botulinum types A & E C. perfringens / C. histolyticum C. tertium / C. bifermentans C. sporogenes Corynebacterium bovis Escherichia coli E. coli O157:H7 Helicobacter pylori Lactobacillus plantarum Legionella pneumophila Listeria monocytogenes Pseudomonas aeruginosa Pseudomonas fluorescens Salmonella typhimurium Salmonella paratyphi B Salmonella derby Salmonella stanley Staphylococcus aures Streptococcus lactis Strep. dysgalactiae / Strep. uberis Yersinia enterocolitica Antiviral activity Polio virus type I Human adeno virus Simian virus 40 / Kilham rat virus Coxasackie virus CB3 & CB5 Human immunodeficiency virus Human rotavirus Hepatitis A virus Antiparasitic activity Cryptosporidium parvum Giardia sp.
Free chlorine
Contact time
Reference
0.01 ppm n/a n/a 100 ppm 7.5 ppm 200 ppm 5 ppm 0.1 mg 4.5 ppm 5 ppm 5 ppm 5 ppm n/a 12.5 ppm 2000 ppm n/a 5.0 ppm 0.1 mg 2000 ppm 25 ppm 25 mg/ml n/a 50 mg/L 0.02 ppm 12.5 ppm 0.1 mg/ ml 1 g/L 6 ppm n/a 10 mg/L 500 ppm
5 min n/a n/a 5 min / 60 min 8 min 9 min 27 min 5 min 10.5 & 6.0 min 60 min / 10 min 20 min 35 min n/a 15 sec 1 min n/a 15 sec 40 min 1 min n/a 2 hours n/a 1 min 5 min 15 sec 5-10 min n/a 15 sec n/a 120 sec n/a
Ridenour & Ingols, 1947 Sisti et al., 1998 Greene et al., 1993 Cousins & Allan, 1967 Seeger, 1978 Seeger, 1978 Labree et al., 1960 Blaser et al., 1986 Ito & Seeger, 1980 Dye & Mead, 1972 Dye & Mead, 1972 Dye & Mead, 1972 Oliver et al., 1989 Mosley et al., 1976 Beuchat et al., 1998 Johnson et al., 1997 Hays et al., 1967 Kuchta et al., 1983 Beuchat et al., 1998 Lin et al., 1996 Samrakandi et al., 1997 Greene et al., 1993 Williams et al., 1990 Ridenour & Ingols, 1947 Mosley et al., 1976 Jaquette et al., 1996 King et al., 1977 Hays et al., 1967 Oliver et al., 1989 Paz et al., 1993 Escudero et al., 1999
0.03 mg/L 0.3 - 0.6 mg/L 1 mg/L n/a n/a 50 ppm 0.5 mg/L n/a 0.5 - 1.0 mg/L
n/a 15-30 min n/a n/a n/a 2 min n/a n/a n/a
Thraenhart & Kuwert, 1975 Carlson et al., 1976 Abad et al., 1994 Engelbrecht et al., 1980 Jensen et al., 1980 Bloomfield et al, 1990 Abad et al., 1994 Grabow et al., 1983 Abad et al., 1994
0.4 mg/L n/a
15 min n/a
Peeters et al., 1989 Haas & Aturaliye, 1999
(n/a, data not available)
elevated (39 to 40˚C) temperatures in filtered well water (pH 7.3) for their efficacy in inactivating Legionella pneumophila ATCC 33155 (Landeen et al., 1989). At room temperature, a contact time of at least 24 h was necessary for copper and silver (400 and 40 µg/L) to achieve a 3-log10 reduction in bacterial numbers. As the copper and silver con-
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centration increased to 800 and 80 µg/L, the inactivation rate significantly increased from K = 2.87 x 10-3 to K = 7.50 x 10-3 (log10 reduction per minute). In water systems with and without copper and silver (400 and 40 µg/L), the inactivation rates significantly increased as the free chlorine concentration increased from 0.1 mg/L (K = 0.397 log10 reduction per min) to 0.4 mg/L (K = 1.047 log10 reduction per min). Compared to room temperature, no significant differences were observed when 0.2 mg of free chlorine per liter with and without 400 and 40 µg of copper and silver per liter was tested at 39 to 40˚C. All disinfection systems, regardless of temperature or free chlorine concentration, showed increase inactivation rates when 400 and 40 µg of copper and silver per liter was added; however, this trend was significant only at 0.4 mg of free chlorine per liter. Orth and Mrozek (1989) evaluated the effectiveness of sodium hypochlorite against a number of pathogenic organisms, including L. monocytogenes, Campylobacter jejuni, and Yersinia enterocolitica. The results indicated that different organisms were destroyed by chlorine under practical use conditions of time, temperature, and concentration. However, certain strains displayed varying degrees of resistance to chlorine. Campylobacter jejuni and closely related organisms are important bacterial causes of acute diarrheal illness. Both endemic and epidemic infections have been associated with consuming untreated or improperly treated surface water. Blaser et al. (1986) compared susceptibility of three C. jejuni strains and E. coli with standard procedures used to disinfect water. Inactivation of bacterial preparations with 0.1 mg of chlorine and 1.0 mg of monochloramine per liter was determined at pH 6 and 8 and at 4 and 25˚C. Under virtually every condition tested, each of the three C. jejuni strains was more susceptible than the E. coli control strain, with greater than 99% inactivation after 15 min of contact with 1.0 mg of monochloramine per liter or 5 min of contact with 0.1 mg of free chlorine per liter. Results of experiments in which an antibiotic-containing medium was used suggest that a high proportion of the remaining cells were injured. An animal-passaged C. jejuni strain was as susceptible to chlorine disinfection as were laboratory-passaged strains. These results suggest that disinfection procedures commonly used for treatment of drinking water to remove coliform bacteria are adequate to eliminate C. jejuni and further correlate with the absence of outbreaks associated with properly treated water. The effects of chlorine at varying pH, culture media and incubation temperatures on one type and two wild type strains of Yersinia enterocolitica were studied (Paz et al., 1993). Exposure to 1 and 5 mg/L did not diminish viability, even after prolonged exposure. A level of 10 mg/L was required to achieve a 5-log reduction in 120 s for the type strain and 80 s for the wild strains. There was an increase of more than 30% in the rate of disinfection with a 10˚C rise, a remarkable increase in antimicrobial activity at pH 5-log reduction in 20 s, as well as marked neutralization of the effect in the presence of 0.1% peptone. Cells at exponential growth-phase were more susceptible than stationary-phase ones. Cells from liquid medium were more resistant than those from solid medium. Johnson et al. (1997) demonstrated that Helicobacter pylori was readily inactivated by free chlorine and suggested the control of this gastric pathogen by disinfection practices normally employed in the treatment of drinking water. The susceptibility of toxigenic Aeromonas spp. to free chlorine in drinking water supplies, and the influence of environmental temperature on the bactericidal activity of the oxidant, were evaluated (Sisti et al., 1998). The inactivation curves were characterized by an initial phase of rapid reduction of viable cells followed by a slow inactivation of bac-
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FIGURE 2. Antimicrobial activity of chlorine dioxide against E.coli and B. subtilis. Inactivation of E.coli cells in aqueous suspension at ClO2 concentrations (mg/L): 0.7 (❍); 1.4 (); 2.8 ( ); and 3.5 () (redrawn from Foschino et al., 1998). Sporicidal kinetics of ClO2 gas sterilization in ambient humidity - B. subtilis ssp. niger cells were exposed to 7 (); 15 () or 30 () mg/L of ClO2 gas under square-wave conditions at 23°C (redrawn from Jeng & Woodworth, 1990).
teria. The effect of a chlorine compound is markedly influenced by water temperature. At summer water temperature (20˚C), the efficacy of the chlorine concentrations tested was found two to three times lower compared to that found at a winter temperature (5˚C). Resistance was higher in A. hydrophila than A. caviae and A. sobria, but all Aeromonas spp. were more susceptible than E. coli. Selective pressure with free chlorine did not produce Aeromonas cells with higher levels of chlorine resistance. The efficacy of ClO2 against cells of E. coli in aqueous suspension and adhering to the surfaces of stainless steel AISI 304 and PVC was evaluated (Foschino et al. 1998). The concentrations tested ranged from 0.7 to 14 mg/L; at 30s and 1, 2, 4, and 8 min exposure times. When the bacteria were suspended in water with 1.4 mg/liter of ClO2, a 5-log reduction occurred within 30s (FIGURE 2); when cells were attached to the steel surface, similar inactivation took place only after 6 min with 7 mg/L or 4 min with 14 mg/L of ClO2. A 5-log reduction was not obtained when organisms adhered to polyvinyl chloride (PVC). Effect of chlorine and ozonation on E. coli cells resuspended in wastewater was compared (Arana et al., 1999). Selected chlorination and ozonation conditions produced a similar decrease in viability (2-2.5 log). Under such conditions, differences in membrane permeability and cell surface hydrophobicity were detected, depending on the disinfectant tested. No changes in cell surface hydrophobicity were observed after ozonation, however, approximately 95.5% of cells showed altered membrane permeability. The effect of chlorine was not linked to changes in membrane permeability. After chlorination, E. coli cells showed a tendency to aggregate. The degree of toxicity was unrelated to the effect on cellular activity.
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B. Antiviral activity Different types of enteric viruses show marked variations in the degree of resistance to free chlorine. Poliovirus, coxsackievirus, and some echoviruses are more resistant than coliform or enteric pathogenic bacteria (Dunham, 1977; Kabler et al., 1961). Poliovirus type I is a highly stable pathogen in drinking-water and sewage lines. Thraenhart and Kuwert (1975) evaluated a comparative inactivation of poliovirus type I strains (wild type and attenuated) with chlorine and ozone treatments. Defined quantities of disinfectants were examined for viral inactivation in water without redox-potential (double-distilled water), water with low defined redox-potential (double-distilled water + KOH), previously chlorinated water with a residual chlorine content of 0.03 mg chlorine per liter (tap water) and water with a high redox-potential (well water from the drinkingwater plant). Time-course studies were performed, with both chlorine and ozone, in order to evaluate the characteristics of the inactivation procedure. Chlorine and ozone demonstrated similar virus-disinfection profile. The initial rate and kinetics of virus disinfection were identical. The antiviral activities of both disinfectants were dependent on redoxpotential and pH of the water. In contrast to the amount of free chlorine, the value of the oxidation-reduction potential (ORP) was found to be a criterion of virus inactivation (Carlson et al., 1976). For virus inactivation, higher ORP values and longer periods of contact was necessary than for the killing of bacteria. To ensure the inactivation of poliovirus in water contaminated with organic substances, an ORP of +780 mV (0.3-0.6 mg/L free chlorine) should be maintained for 15-30 min. Adenovirus also demonstrated similar resistance to inactivation. The rate of inactivation of poliovirus in water by chlorine is strongly influenced by the pH, which in turn influences the relative amounts of HOCl and OCl- that are present and acting on the virus in the region of pH 6 to 10. The distribution of HOCl and OCl- is influenced to a lesser extent by the addition of NaCl. The major part of the sharp increase in disinfection rate seen with this salt is thought to be due to its effect on the virus itself resulting in an increased chlorine sensitivity, especially at high pH (Sharp et al., 1980). ClO2, bromine chloride and iodine were compared with chlorine as virucidal agents (Taylor & Butler, 1982). Under optimal conditions, all disinfectants were effective at low concentrations, but each disinfectant responded differently to acidity and alkalinity. Disinfection by chlorine was impaired by the presence of ammonia, but the other disinfectants retained much of their potency. Disinfection of poliovirus by iodine resulted in structural changes in the virions as seen by electron microscopy, but the other disinfectants were able to inactivate poliovirus without causing any apparent structural changes. Berg et al. (1989) reported a rapid inactivation of poliovirus by free chlorine at 5 ˚C and pH 9 in drinking water. Different ions from many salts present in the water seem to potentiate the virucidal activity of chlorine. The kinetics of inactivation of six enteric viruses, simian virus 40 and Kilham rat virus by free available chlorine under controlled laboratory conditions was reported (Engelbrecht et al., 1980). Different virus types demonstrated a wide range of susceptibility to chlorine disinfection. The rate of inactivation was greater at pH 6 than at pH 10; however, the relative susceptibilities of the viruses were affected differently by a change in pH. The presence of potassium chloride also affected the susceptibility of viruses to chlorine. The inactivation rates of coxsackievirus B3 (CB3) and B5 (CB5) by chlorine in dilute buffer at pH 6 were comparable and about half that of poliovirus (Mahoney) under similar conditions (Jensen et al., 1980). Purified CB3, like the poliovirus, aggregated in
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the acid range but not at pH 7 and above. Purified CB5 aggregated rapidly at all the pH values tested. Addition of 0.1 M NaCl to the buffer at pH 6 did not influence the aggregation of CB5 or the rate of chlorine action on either of the coxsackie-viruses, but at pH 10, the disinfection activity of OCl- for both viruses was increased by 20-fold. Cesium chloride had a similar but smaller effect. KCl was the most active causing inactivation of OCl- at pH 10 about equal to that of HOCl at pH 6. In a study by Grabow et al. (1983). hepatitis A virus (HAV) and selected indicator organisms were mixed together in chlorine-demand-free buffers at pH 6, 8, or 10 and exposed to free chlorine residuals and the survival kinetics of individual organisms were compared. HAV was enumerated by a most-probable-number dilution assay, using PLC/PRF/5 liver cells for propagation of the virus and radioimmunoassay for its detection. At all pH levels, HAV was more sensitive than Mycobacterium fortuitum, coliphage V1 (representing a type of phage common in some sewage-polluted waters), and poliovirus type 2. Under certain conditions, HAV was more resistant than E. coli, Streptococcus faecalis, coliphage MS2, and reovirus type 3. It remained more resistant than SA-11 rotavirus. However, conditions generally specified for the chlorine disinfection of drinking-water supplies effectively inactivated HAV. Using a quantitative suspension test method, the antiviral activity of sodium hypochlorite (NaOCl) and sodium dichloroisocyanurate (NaDCC) against human immunodeficiency virus (HIV) was investigated (Bloomfield et al., 1990). Viral suspensions were prepared containing 104-105 syncitial forming units/ml in 0.9% saline or 0.9% saline containing 10% v/v plasma to simulate clean and dirty conditions. A syncitial inhibition assay on C8166 lymphoblastoid line was performed to determine viral titer. Results indicate that satisfactory disinfection (3-4 log reduction in 2 min) could be achieved with NaDCC and NaOCl at concentrations of 50 ppm and 2500 ppm available chlorine for clean and soiled conditions, respectively. For treatment of blood spillage, the addition of NaDCC and NaOCl solutions (10,000 ppm) to equal volumes of contaminated blood (giving a final available chlorine concentration of 5000 ppm of blood) was sufficient to produce total kill within 2 min. For treatment of spillage material, chlorine-releasing powder formulations that produce higher available chlorine concentrations and achieve containment of spillage material offer an effective alternative. The efficacy of copper and silver ions, in combination with low levels of free chlorine (FC), was evaluated for the disinfection of hepatitis A virus (HAV), human rotavirus (HRV), human adenovirus, and poliovirus (PV) in water (Abad et al., 1994). HAV and HRV showed little inactivation in conditions tested. PV showed more than a 4 log10 titer reduction in the presence of copper and silver combined with 0.5 mg of FC per liter or in the presence of 1 mg of FC per liter alone. Human adenovirus persisted longer than PV with the same treatments, although it persisted significantly less than HRV or HAV. The addition of 700 µg of copper and 70 µg of silver per liter did not enhance the inactivation rates after the exposure to 0.5 or 0.2 mg of FC per liter, although on some occasions it produced a level of inactivation similar to that induced by a higher dose of FC alone. Virus aggregates were observed in the presence of copper and silver ions, although not in the presence of FC alone. Chlorine compounds have demonstrated cidal activity against bacteriophage. Sing et al. (1964a, b) compared the destructive activity of several germicidal aerosols against Streptococcus cremoris phage 144F. The levels of 500-2000 ppm available chlo-
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rine were highly effective against bacteriophage on a variety of surfaces. McCoy and Irwin (1974) examined the effect of various disinfectants on E.coli phage →X174 and found similar concentrations of chlorine to be effective. Finichiu et al. (1986) studied the resistance of different microorganisms to chlorine to assure good drinking water quality and concluded that the resistance of bacteria to chlorine was much lower than that of viruses. C. Antifungal activity The fungicidal activity of chlorine has not been as extensively investigated as its bactericidal or sporicidal activity. Cheng and Levin (1970) studied the inactivation of Aspergillus niger conidiospores in the presence of 1-20 ppm chlorine. Fungal spores are slightly more resistant than vegetative bacteria since the germicide must mobilize farther to penetrate the coat of a fungal spore compared to a vegetative cell. Ver Kuilen and Marth (1980) reported the sporicidal effect of hypochlorite on Aspergillus parasiticus. Brown and Wardowski (1986) reported the use of chlorine in citrus packaging houses for the reduction of decay on citrus fruits caused by Penicillium digitatum and Geotrichum candidum. The use of chlorine or ClO2 under different plant conditions demonstrated an effective control of these organisms. Although 0.4% chlorine for 2 min has been recommended for surface disinfection of food samples before direct plating for fungal enumeration, this procedure may not be adequate for highly contaminated products. The effectiveness of a range of chlorine solutions was investigated using barley samples artificially contaminated with four different concentrations of Aspergillus flavus. A. niger, A. ochraceus, Eurotium repens, Penicillium brevicompactum, P. chrysogenum and Cladosporium cladosporioides (Andrews et al., 1997). At initial contamination levels >104/g, 0.4% chlorine did not inactivate sufficient spores to produce less than 20% contamination. Of the test fungi, ascospores of E. repens were the most resistant to chlorine inactivation, whereas the conidia of C. cladosporioides were the most susceptible. D. Sporicidal activity The sporicidal activity of some of the organic chlorine compounds was reviewed by Trueman (1971). For trichloroisocyanuric acid, the sporicidal activity was significantly lower, although comparable, if not superior, results were obtained against sensitive vegetative bacteria compared to hypochlorite. Chloramine is also less sporicidal than hypochlorite (Odlaug, 1981). Dichloroisocyanuric acid was found to be comparable, to sodium hypochlorite in the destruction of bacteriophage (Sing et., 1964a, 1964b). Trichloroisocyanuric acid has also been shown to inactivate bacteriophage at low levels (10 ppm) in aqueous solution (Fortney, 1958). Sodium and potassium hypochlorites may be used on some polymeric and metallic membranes. Because of material restrictions, only a few types of membranes are compatible with chlorine, but even these require restrictions of temperature, concentration, pH, and exposure time. Bragulla and Liutner (1987) suggested the use of chlorine on different membranes and some of its limitations. Russel (1990) showed that active chlorine compounds are not only bactericidal but also sporicidal. Hypochlorites in combination with sodium hydroxide were found more efficient sporicidal mixtures than by themselves.
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E. Antiparasitic activity Effect of disinfection of drinking water with ozone or chlorine dioxide on survival of Cryptosporidium parvum oocysts was reported (Peeters et al., 1989). Preliminary trials indicated that a minimum infection level of 1,000 oocysts (0.1-ml inoculum) per mouse was necessary to induce 100% infection. Treatment of water containing 104 oocysts per ml with 1.11 mg of ozone per liter (concentration at time zero [C0]) for 6 min totally eliminated the infectivity of the oocysts for neonatal mice. A level of 2.27 mg of ozone per liter (C0) was necessary to inactivate water containing 5 x 105 oocysts per ml within 8 min. Also, 0.4 mg of ClO2 per liter (C0) significantly reduced infectivity within 15 min of contact, although some oocysts remained viable. The effect of electroporation (pulses of high voltage electricity for very short duration) on the viability of Giardia cysts and Cryptosporidium oocysts, and on the viability of these organisms in the presence of free chlorine, combined chlorine, hydrogen peroxide and potassium permanganate, was examined (Haas & Aturaliye, 1999). While electroporation itself had only a minor effect on survival, the combination of electrical and chemical treatment produced superior inactivation, particularly with combined chlorine, hydrogen peroxide and potassium permanganate. This enhancement may provide a practical way of achieving enhanced inactivation of resistant protozoa by water disinfection processes.
V. APPLICATIONS Among the various sanitizers used in the industry today, such as quaternary ammonium salts, ozone, iodophores, gluteraldehyde, and ethylene oxide, chloro-cides have the largest market-share. The key features of these compounds that have made them a popular choice are: 1) high antimicrobial efficacy, 2) low toxicity to humans, 3) versatile application, 4) ease of use, 5) low-cost, and 6) safe handling. Some of the drawbacks of chloro-cide use that are faced in the industry today are related to their irritant nature and their corrosive potential. Nevertheless, these problems could be circumvented by following appropriate directions for use and by adding anti-corrosion agents. The commonly used salt additives that diminish metal corrosion are nitrates, phosphates, disodium phosphate or sodium pyrophosphates. Corrosion can be prevented with 0.5 to 4 g/L of acid or neutral form of tartrates (Na, K or NH4), or organic amino compounds such as amines, amides or heterocyclic bases (Masschelein, 1979). Chlorine in its various forms is the most widely used chemical sanitizer in the food industry. In general, the organo-chlorines are slower acting bactericides than the inorganic forms, but they offer the advantage of stability and are relatively less irritating to personnel and less corrosive to equipment. Chlorine compounds are utilized: As adjuncts to water used for conveying raw food products, as well as water used for cooling of heat-sterilized cans. As sanitizing solution for food contact surfaces. In the treatment of raw meat, poultry, and fish to reduce microbial load and to extend shelf life. The following Section describes the specific applications of chloro-cides in different industry sectors.
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A. Dairy sanitation The efficacy of chlorine disinfectant on teats artificially contaminated with a milk suspension of Staphylococcus aureus was reported (King et al., 1977). A solution of sodium hypochlorite with 40 g/L available chlorine was significantly more bactericidal than one containing 1 g/L available chlorine and more bactericidal than most other disinfectants tested. However, there were no distinguishable differences in efficacy between solutions containing 40 g/L and 10 g/L available chlorine and some of the iodophors containing 5 g/L available iodine. The addition of 190-416 g/L (15-33% v/v) glycerol significantly reduced the bactericidal properties of 3 iodophors (5 g/L available iodine), but soluble lanolin at approximately 20 g/L did not appear to lower the efficiency of sodium hypochlorite (45 g/L available chlorine) or of an iodophor (5 g/L available iodine). Ozonated water and chlorinated sanitizer were compared for effectiveness against biofilms of milk spoilage bacteria (Greene et al., 1993). Stainless steel plates were incubated in UHT-pasteurized milk inoculated with pure cultures of either Pseudomonas fluorescens or Alcaligenes faecalis. Both ozonation and chlorination reduced bacteria populations by > 99% at initial cell densities in the range of approximately 1.24 x 105 to 8.56 x 105 cfu/cm2 for P. fluorescens and 1.53 x 104 to 8.56 x 105 cfu/cm2 for A. faecalis in milk films on stainless steel surfaces. Chlorine and monochloramine show an equal biocidal activity on lactose medium-grown E. coli and glycerol-ammonium nitrate medium-grown nonmucoid Pseudomonas aeruginosa biofilms (Samrakandi et al., 1997). In contrast, the effect of monochloramine is greater compared with that of chlorine on E. coli and mucoid P. aeruginosa biofilms grown in sucrose and glycerol-ammonium nitrate media, respectively. In these culture conditions, treatment with 25 mg monochloramine/L for 2 h reduced viable cells by 4.5 logs for E. coli and about 3 logs for mucoid P. aeruginosa while the similar treatment with chlorine reduced viable cells by 4.5 logs for E. coli and about 3 logs for mucoid P. aeruginosa while the similar treatment with chlorine reduced viable cells in these biofilms by 2.2 logs and 1 log, respectively. The decrease of chlorine disinfection efficacy on sucrose and glycerol-ammonium nitrate medium-grown biofilms is postulated to be linked to the higher polysaccharide production observed in these media. It seems likely that monochloramine produces a high leakage of material absorbing at 260 nm from sucrose medium-grown E. coli biofilm, which could indicate its better penetration into biofilms. Prevention of bovine mastitis by a postmilking teat disinfectant containing chlorous acid and chlorine dioxide in a soluble polymer gel was reported by Oliver et al. (1989). A natural exposure study was conducted in a herd of 150 lactating dairy cows for 18 months to determine the effectiveness of chlorous acid and chlorine dioxide in a soluble polymer gel as a postmilking teat disinfectant for the prevention of bovine mastitis. Right quarters of cows were dipped in the experimental teat dip after milking machine removal. Left quarters were not dipped and served as within-cow negative controls. The experimental teat dip reduced Staphylococcus aureus infections 67.4%, Streptococcus dysgalactiae infections 63.8%, and Streptococcus uberis infections 27.8%. Overall efficacy of the chlorous acid and chlorine dioxide teat dip against major mastitis pathogens was 52.2%. The experimental teat dip reduced Corynebacterium bovis infections and coagulase-negative staphylococcal infections also by 45.8 and 38.7%, respectively. Overall efficacy against minor mastitis pathogens was 43.4%. Under conditions of this trial, the experimental teat dip containing chlorous acid and chlorine dioxide was effective in preventing new intramammary infections against a variety of mastitis pathogens.
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B. Beef and poultry sanitation The Food and Drug Administration has recently approved the use of acidified sodium chlorite solutions for the decontamination of red meat carcasses and poultry (FDA, 1998). Castillo et al., (1999) studied the effect of acidified sodium chlorite on beef carcasses that were inoculated with Escherichia coli O157:H7 and Salmonella typhimurium. The sodium chlorite solutions were activated with phosphoric or citric acid, and were applied on the carcasses as spray wash subsequent to a water wash. The initial numbers for both pathogens were reduced by 3.8 to 3.9 log cycles when a phosphoric acid activated sodium chlorite was used. The reduction in pathogen count was 4.5 to 4.6 log cycles when a citric acid activated sodium chlorite solution was used. The study concluded that acidified sodium chlorite sprays are very effective for decontaminating beef carcass surfaces. The study also demonstrated that the choice of acid used for the activation of sodium chlorite can have a significant influence on the biocidal activity of this sanitizer. The efficacy of ClO2 as an alternative sanitizing agent for hatching eggs was investigated to overcome health risks with formaldehyde fumigation (Patterson et al., 1990). Hatchability of chicken eggs was reduced when the eggs were dipped in the ClO2 solutions for more than 5 minutes or in concentrations greater than 100 ppm chlorine. However, treatment of hatching eggs with a ClO2 foam or fumigating with formaldehyde had no adverse effect on hatchability compared with untreated control eggs. Sanitizing soiled duck eggs with ClO2 foam improved hatchability by more than 10% and hatch by more than 6% compared with untreated eggs. A novel method for assessing bactericidal potential of egg-sanitizing agents was developed. Using this technique, both chlorine dioxide foam and formaldehyde fumigation reduced the number of egg-contaminant bacteria inoculated on sterile chicken eggs compared with the number of bacteria on untreated eggs. These findings suggested that sanitizing hatching eggs with ClO2 foam might be a viable alternative to fumigating with formaldehyde. Three organic N-halamine compounds (combined halogen disinfectants) were compared with free chlorine (as calcium hypochlorite) as bactericides against Salmonella typhimurium and unidentified normal poultry bacterial flora under controlled conditions of pH, temperature, and halogen demand similar to those encountered in poultry processing (Williams et al., 1990). Two of the compounds (3-chloro-4,4-dimethyl-2-oxazolidinone and 1,3-dichloro-4,4,5,5-tetramethyl-2-imidazolidinone) at a concentration of 50 mg/L were found to cause a significant decline in viable organisms in less than 1 min at 48 °C, whereas a third compound (1-bromo-3-chloro-4,4,5,5-tetramethyl-2-imidazolidinone) was found to be less suitable. C. Produce sanitation According to the US National Advisory Committee on Microbiological Criteria for Foods, in the past two decades there has been a considerable increase in the consumption of fresh fruits and vegetables in the world (Roever, 1999). In the US, there has been a 432% increase in the average number of commodities offered for sale in supermarket produce departments. Subsequently, the occurrence of foodborne illnesses from these foods has also gone up. Therefore, effective compounds for the sanitation of produce are needed. Chlorine has been used as a disinfectant in wash, spray and flume waters in the raw fruit and vegetable industry. To disinfect produce, chlorine is commonly used at con-
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centrations of 50-200 ppm with a contact time of 1-2 minutes. Maximum solubility of chlorine is achieved in water at about 4˚C. However, the temperature of the chlorinated water should ideally be at least 10˚C higher than that of fruits or vegetables to achieve a positive temperature differential, thereby minimizing the uptake of wash-water through stem tissues (Bartz & Showalter, 1981; Zhuang et al., 1995) and open areas in the skin or leaves, whether due to mechanical assault or natural presence (e.g. lenticels and stomata). Elimination of uptake of wash-water that may contain microorganisms, including those that may cause human illnesses, should be considered as a critical control point in handling, processing and disinfection of raw fruits and vegetables. The possible use of chlorinated water in packing-houses and during washing, cooling and transport for the purpose of controlling post-harvest diseases of fruits and vegetables has also been suggested (Eckert & Ogawa, 1988). The effects of chlorine concentration on aerobic microorganisms and fecal coliforms present on leafy salad greens was studied by Mazollier (1988). Populations of pathogens were markedly reduced with increased concentrations of chlorine to 50 ppm, but further increases in concentration to 200 ppm did not have a substantial additional effect. A standard procedure for washing lettuce leaves in tap water reduced population (ca. 107/g) of microflora by 92% (Adams et al., 1989). Inclusion of 10 ppm chlorine (pH 9.0) reduced the count by 97.8%, indicating that this concentration of chlorine in treatment water was only slightly more effective than using water with no chlorine. The pH adjustment from 9.0 to 4.5-5.0 with inorganic and organic acids resulted in a 1.5-4.0-fold increase in microbicidal effect. Increasing the washing time in hypochlorite solution from 5 to 30 minutes did not decrease numbers of microbes further, whereas extended washing in tap-water resulted in a reduction comparable to hypochlorite. Addition of 100 ppm of a surfactant (Tween 800) to hypochlorite washing solution enhanced lethality by enhancing surface contact but adversely affected sensory qualities of lettuce. Somers (1963) reported that wash-water with about 5-ppm chlorine reduced microbial populations on several fruits and vegetables by 57˚C reduced populations to < 1 CFU/g. However, treatment at > 54˚C for 10 min caused a substantial reduction in viability of the seeds. Treatment at 57 or 60˚C for 5 min appears to be effective in killing S. stanley without substantially decreasing germination ability of seeds. Storage of seeds for 8 to 9 weeks at 8 and 21˚C resulted in reductions in populations of S. stanley of about 1 log10 and 2 log10 CFU/g, respectively. The behavior of S. stanely on seeds during soaking, germination, sprouting, and refrigerated storage of sprouts was determined. An initial population of 3.29 log10 CFU/g increased slightly during 6 h of soaking, by about 103 CFU/g during a 24-h germination period, and by an additional 10 CFU/g during a 72-h sprouting stage. A population of 107 CFU/g of mature alfalfa sprouts was detected throughout a subsequent 10-day storage period at 5˚C. These studies indicate that while populations of S. stanley can be greatly reduced, elimination of this organism from alfalfa seeds may not be reliably achieved with traditional disinfection procedures. If S. stanley is present on seeds at the initiation of the sprout production process, populations exceeding 107 CFU/g can develop and survive on mature sprouts exposed to handling practices used in commercial production and marketing.
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In another study, alfalfa sprouts inoculated with a five-serovar mixture of Salmonella (S. agona, S. enteritidis, S. hartford, S. poona, and S. montevideo) were dipped in 200,500 or 2000 ppm chlorine solutions for 2 minutes (Beuchat, 1997). The pathogen was reduced by about 3.4 log10 CFU/g after treatment with 500 ppm chlorine and to an undetectable level (100 ppm
A. hydrophila/ B. subtilis/ E. coli/ V. cholerae/ P.aeruginosa/ L. monocytogenes/ Salm. typhi/ Staph. aureus / Y. enterocolitica Alcaligens faecalis/ P. fluorescens P. putida/ B. thermospacta/ L. plantarum / Shewanella putrefaciens/ Enterobacter sp. Enterococcus seriolicida Pasteurella piscicida/ Vibrio anguillarum E.coli/ Salmonella typhimurium Salmonella sp./ Enterobacteriaceae HVJ virus/ TME virus/ Reo type 3 virus/ murine hepatitis virus Shelf life extension Shelf life extension Shelf life extension Botrytis cinerea/ Scerotinia sclerotiorum 3-6 log reduction of microbial load Botrytis cinerea E.coli O157:H7
Potatoes Cabbage Carrot Peppercorn Black berries Media
20-25 mg/m3 7-13 mg/m3 5-15 mg/m3 60 µl/L 6.7 mg/L 0.3 ppm 3-18 ppm
Greene et al., 1993 Silva et al., 1998 Sugita et al., 1992 Sugita et al., 1992 Chen et al., 1992 Bailey et al., 1996 Sato et al., 1990 Enshina & Voitik, 1989 Enshina & Voitik, 1989 Enshina & Voitik, 1989 Liew & Prange, 1994 Zhao & Cranston, 1995 Barth et al., 1995 Byun et al., 1998
cytochromes in the milk fat globule membrane may serve as focal points for initiation of lipid peroxidation by catalyzing homolytic scission of peroxides (Korycka-Dahl & Richardson, 1980). The effect of ozone stress on polyamine metabolism and membrane lipid peroxidation in lentil seedlings through the amine oxidase and lipoxygenase activity and expression has been investigated (Maccarrone et al., 1997). Ozone could control the expression of these enzymes at the transcriptional level, down-regulating the amine oxidase gene and up-regulating the lipoxygenase gene. The decrease of amine oxidase activity was correlated with the increase of putrescine concentration in the ozone-treated plantlets, whereas the increase of lipoxygenase activity was paralleled by enhanced membrane lipid peroxidation.
V. ANTIMICROBIAL SPECTRUM Ozone is a potent antimicrobial system that could elicit a broad-spectrum of cidal activity on a variety of microorganisms including bacteria, viruses and fungi (TABLE 1). This property has found applications of ozone system in a wide array of public and commercial sanitation processes. A. Antibacterial activity Ozone and chlorine are agents that disinfect by destroying, neutralizing or inhibiting the growth of pathogenic microorganisms. Korol et al. (1995) compared the efficacy of ozone and chlorine treatment of water and its antimicrobial spectrum on a variety of bacterial pathogens. The treatment of drinking water with ozone has shown to be more efficient against spores of Bacillus subtilis. It was observed that the ozone already in dose of 0.35 mg/L produced the reduction of at least 5 log in populations of approximately 106 cells/ml of E. coli, Vibrio cholerae, Salmonella typhi, Yersinia enterocolitica,
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Pseudomonas aeruginosa, Aeromonas hydrophila, Listeria monocytogenes and Staphylococcus aureus. With a dose of 0.50 mg/L of chlorine, the reduction was much smaller for the tested microorganisms (except Vibrio cholerae), while the effect of 2 mg/L of chlorine was similar to the ozone treatment. For spores of Bacillus subtilis, the reduction observed with ozone concentrations of 0.35 and 0.70 mg/L was of almost 3 log, while no considerable effect was obtained with chlorine in the tested conditions. These results have indicated that both disinfectants were consumed during the treatment period, probably because of the water demand and the added bacterial mass. The ability of ozone to disinfect spores of Bacillus spp. and Clostridium spp. has been reported (Foegeding, 1985). The antimicrobial effects of ozonated water in a recirculating concurrent reactor were evaluated against four gram-positive and four gram-negative bacteria, two yeasts, and spores of Aspergillus niger (Restaino et al., 1995). More than 5-log units each of Salmonella typhimurium and Escherichia coli cells were killed instantaneously in ozonated water with or without addition of 20 ppm of soluble starch. In ozonated water, death rates among the gram-negative bacteria (S. typhimurium, E. coli, Pseudomonas aeruginosa, and Yersinia enterocolitica) were similar. Among gram-positive bacteria, Listeria monocytogenes was more sensitive than Staphylococcus aureus or Enterococcus faecalis. In the presence of organic material, death rates of S. aureus compared with L. monocytogenes and E. coli compared with S. typhimurium in ozonated water were not affected by addition of soluble starch but were markedly reduced by addition of 20 ppm of bovine serum albumin. More than 4.5-log units each of Candida albicans and Zygosaccharomyces bailii cells were killed instantaneously in ozonated water, whereas 99% at initial cell densities in the range of approximately 1.24 to 8.56 x 105 CFU/cm2 for P. fluorescens and 1.53 x 104 to 8.56 x 105 CFU/cm2 for A. faecalis in milk films on stainless steel surfaces. The bactericidal activity of gaseous ozone was examined on five species of fish bacteria, Pseudomonas putida, Shewanella putrefaciens, Brochothrix thermospacta, Enterobacter sp., and Lactobacillus plantarum (Silva et al., 1998). Test strains were inoculated on agar surfaces and exposed to different ozonation times in a gas chamber. Relatively low concentrations ( 100 ppm) at high humidity was highly virucidal against four RNA viruses including HVJ, Theiler’s murine encephalomyelitis virus (TMEV), Reo type 3 virus (RV) and murine hepatitis virus (MHV). Antiviral tests with ozone were performed with 0.1 ml of virus suspension in deionized water or saline, placed in 35-mm dishes. The titer of 106 plaque-forming units of TMEV in a liquid-phase, which was highly stable against physical treatments, was reduced within 1 h to a level of 0 by 300 ppm of ozone at 80% humidity and 22-25˚C. HVJ and MHV were more susceptible than TMEV to the ozone treatment. RV was the most resistant of the 4 viruses tested. The authors suggested that ozonation is a promising method to disinfect not only the laboratory animal RNA-viruses (both of enveloped and non-enveloped viruses) but also animal rooms, clean rooms and safety cabinets.
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VI. APPLICATIONS In recent years, ozone technology has found uses in agriculture and the food industry; however, it has been used in other industrial applications for a long time. The industrial applications of ozone have been focused on ozone’s ability to oxidize and sterilize, without leaving residues. Applications of ozone in the water, wastewater treatment, and food processing appear highly promising. These include preserving raw agricultural commodities during storage and transit, controlling odor, retarding metabolic processes associated with ripening, and sanitizing water utilized for washing food equipment, foods, and packaging materials. A. Treatment of drinking water During the early 1900s, ozone was suggested as a disinfectant for drinking water. Ozone is still used in the disinfection of water supplies in many European countries. Ozone acts with efficacy even at lower concentration under controlled conditions with few known side effects such as taste, odor and toxic by-products. Ozone applications in water treatment can be classified into three types: 1. Disinfection. Ozonation is generally performed at the end of the water treatment process, prior to chemical addition, flocculation, sedimentation and filtration. Such treated water is clean and free of high concentrations of oxidizable organic materials, other than the lysed bacterial cells or inactivated viruses (Rice, 1986). A residual ozone standard for water treatment plants has been adopted first by the French Public Health Authorities. A residual ozone concentration of 0.4 mg/L is recommended for at least 4 minutes and maintained for an additional 4 minutes of contact time. A contact time of 8 minutes has a 99.9% efficacy to inactivate viruses and kill bacteria. In operational drinking water treatment plants, ozone disinfection/viral inactivation normally is accomplished using two or more side-by-side contact chamber. The 4 mg/L level is attained in the first chamber, and is maintained in the second or subsequent chambers. In normal practice, the first four minutes contact time is at least doubled, to eight to 12 minutes, to ensure that the require disinfection conditions are achieved (Rice, 1986). 2. Oxidation. Impurities such as iron, manganese, organic contaminants, phenols, inorganic impurities such as cyanide sulfide and nitrite, instantly react with ozone. It is hard at this point to provide a standard contact time and ozone concentration due to the variability and level of contaminants. Ozonation at this stage normally produces water which is more turbid than the prior treatments. Products from oxidation reaction combines with polyvalent cations, hydrogen bonding and produces higher molecular weight adducts which are insoluble and could be precipitated and removed from the water. 3. Bio-processing. The purpose of water treatment in this case is to increase dissolved oxygen and to oxidize complex organic contaminants for easier degradation. The optimum ozone concentration for this treatment is 1 mg/L per mg/L of organic contaminants (Nagel et al., 1982).
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B. Wastewater treatment Ozone has been successfully used in sewage treatment plants for several decades and in many countries. Fox example, ozone could be used instead of chlorine in the final disinfection process of effluent prior to discharge into a receiving stream. Other applications include pretreatment and odor control of influent (Rice, 1986). C. Food processing The possible formation of carcinogenic compounds in water (Brungs, 1973) has raised questions about the use of certain chlorine compounds in food processing. The food industry is searching for alternative compounds for cooling water and wastewater disinfection. Numerous investigations on disinfection of foods (including the usage of gaseous ozone for shelf life enhancement, ozone dissolved in water for sanitizing surfaces of vegetables, fruits, and other agricultural products) strongly support the idea that ozone is a powerful disinfectant. Ozone has been used in the European food industry for decades, in certain instances for almost a century. However, the food industry in the U.S. has little or no experience with application of ozone to foods. This may be due to lack of studies on the efficacy of ozone in food processing, safety issues, toxicology, and impact on nutrients. Applications for ozone in the food processing/packaging industries are extremely varied (Graham, 1997). Based on potent disinfection and oxidation properties, various possibilities for use of ozone in food industry and agriculture have been developed. There are few published applications of ozone, e.g., cleaning shellfish (Anonymous, 1972), preserving fish (Haraguchi et al., 1969), aflatoxin reduction in peanut and cottonseed meals (Dwankanth, 1968), sterilization of bacon, bananas, butter, eggs, mushrooms, cheese, fruits (Gammon & Kerelak, 1973), and beef (Kaess & Weidemann, 1968a; 1968b), disinfection of poultry carcasses and chill water (Sheldon & Brown, 1986; Bolder, 1997). Sheldon and Brown (1986) investigated the efficacy of ozone as a disinfectant for poultry carcasses. The microbial counts of ozone treated carcasses stored at 4˚C were markedly lower than carcasses chilled under non-ozonated conditions. Ozone also has been evaluated against various sanitizing agents (5% hydrogen peroxide, 0.5% ozone, 12% trisodium phosphate, 2% acetic acid, and 0.3% commercial sanitizer), and water (16 to 74˚C) spray-washing interventions for their ability to reduce bacterial contamination on beef samples in a model spray-washing cabinet (Gorman et al., 1995) Under the conditions of their study, hydrogen peroxide and ozonated water were more effective than other sanitizing agents. However, the study conducted by Reagan et al (1996) on the effects of different treatments (74˚C hot-water washing, 5% hydrogen peroxide, and 0.5% ozone) in reducing bacterial populations on beef carcasses showed that the ozone and hydrogen peroxide treatments had minor effects and were equivalent to conventional washing in reducing bacterial populations on beef. 1. Preservation and storage. Ozone is also being shown effective for increasing the storage life, ranging from minimally processed to fully processed commodities, by reducing the level of food spoilage microorganisms contained on the food surface. The use of ozone has become popular in several major cold storage plants in Europe (Horváth et al, 1985).
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Practical operations for such preservation is based on the sterilization of air entering the storage room contain a sufficient amount of ozone to destroy microorganisms. Billion (1975) conducted a detailed investigation on the storage life of beef, veal, lamb, pork, chicken, and rabbit in ozonated atmospheres. Ozonated atmosphere increased the storage life of all the foods studied by 7 days compared to normal atmosphere. In general the growth of the surface microflora (Pseudomonas sp., spore-formers, salmonellae, and staphylococci) was retarded in refrigerated atmospheres and in the presence of ozone. 2. Effect on odors. Ozone has a characteristic odor, yet the result of application does not mask odors. Atomic oxygen formed by decomposition of ozone immediately oxidize various odor-causing materials. The characteristic putrid odor, however, remains and is difficult to eliminate with ozonation. In general, lower the temperature and larger the molecules in the reaction, weaker is the oxidizing effect. The moisture content in the air has no effect on the process. At very low concentration (0.01 to0.04 ppm ozone), air of the storage facility is felt fresh and pleasant without any stuffy odor. Studies showed that the odor of aromatic fruits such as strawberries is enhanced in the presence of ozone (Gammon & Kerelak, 1973). The formation of fragrances and odors that impart characteristic flavor to fruit is seemed to be enhanced by ozone. The sterilization of air in fruit storage by ozone prevents the odors of packaging materials from transfer to the commodities, a phenomena which frequently takes place otherwise, particularly when wooden crates are used in refrigerated stores at relative humidity of 85% to 90% (Horváth et al., 1985). Storage places, warehouses and refrigerated stores could be disinfected in most cases by administering ozonated air. Besides disinfection, such a process could remove unpleasant odors of packaging materials and could retain the original flavor. The oxidation of compounds creating odors in such premises has the advantage of creating an atmosphere resembling pleasant fresh air. For such purposes, a low concentration of ozone (0.01 to 0.04 ppm) would be sufficient. 3. Effect on metabolism. Effects of ozone on the metabolism is also a consequence of its strong oxidizing ability. No deterioration of fruit is observed, since ozone only affects the surface. During storage, the respiration and ripening process of the fruit is enhanced. Ethylene produced during the storage affects the other fruit and initiates even more intensive ripening. The external signs of this process are the turning brown of the skin, softening of the flesh and, finally, the decay of the fruit. This process is controlled by ozone by the oxidation of metabolic products, thereby reducing the process of back action on other fruits. Moreover, ozone can also promote the healing of wounds and enhance resistance of fruit to infection (Horváth et al., 1985). D. Sanitation of produce The food value of potatoes, cabbage and carrot was studied after ozone treatment to prolong shelf life (Enshina & Voitik, 1989). The regimen of ozone-treatment of the vegetables under laboratory conditions was: 20-40 mg/m3/4-h/day/25 times. Ozone concentration for potatoes treatment was 20-25 mg/m3, cabbage 7-13 mg/m3, carrot 5-15 mg/m3. Ozone treatment did not significantly alter the protein and starch in potatoes; sugar and carotene in cabbage or carrot. Organoleptic evaluation indicated no changes in the properties of potatoes and vegetables as compared to non-treated products. However, ozonation has decreased the ascorbic acid content by 16 to 25%. © 2000 by CRC Press LLC
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Effects of ozone and storage temperature on carrots and two post-harvest pathogens, Botrytis cinerea Pers. and Sclerotinia sclerotiorum de Bary were investigated (Liew & Prange, 1994). Pathogen-inoculated and uninoculated whole carrots were exposed to an ozone concentration of 0 (control), 7.5, 15, 30, or 60 µl/L. Treatment chambers were flushed with a total flow rate of 0.5 liters/min (air and ozone) for 8 h daily for 28 days. The experiment was repeated twice at storage temperatures of 2, 8, and 16˚C. The residual ozone concentration (ozone supplied-exhausted and reacted ozone) increased with ozone supply concentration but was less at higher storage temperatures. A 50% reduction of daily growth rates of both fungi at the highest ozone concentration indicated that ozone is a potent fungistatic system. Carrot respiration rate, electrolyte leakage, and total color differences increased with ozone concentration. Ozone-treated carrots were lighter and less intense in color than control carrots. The use of ozone as a substitute for ethylene oxide to decontaminate whole black peppercorn and ground black pepper and the effects of ozone on the volatile oil constituents of the spice were studied (Zhao & Cranston, 1995). Black peppercorns were immersed in water and sparged with ozonized air (ozone conc., 6.7 mg/L) for 10 min at an air flow rate of 6 L/min. This treatment reduced the microbial population of peppercorn by 3-4 log numbers. Ground black pepper with various moisture levels was sparged with ozonized air for upto 6 h. This treatment reduced the microbial population by 3-6 log numbers, depending on the moisture content of the spice. Higher moisture content led to greater reduction in microbial load. The volatile oil constituents of the spice with and without ozone treatment were extracted with isopropyl ether and analyzed by gas chromatography (GC) and GC-mass spectrometry. Ozone treatment of ground black pepper resulted in the oxidation of certain volatile oil constituents while the treatment had no significant effect on the volatile oil constituents of whole peppercorn. Ozone exposure was assessed for storage of thornless blackberries which are prone to fungal decay (Barth et al., 1995). Blackberries were harvested and stored for 12 days at 2˚C in 0, 0.1. and 0.3 ppm ozone. Berries were evaluated for fungal decay, anthocyanins, color and peroxidase activity. Ozone storage suppressed fungal development for 12 days, while 20% of control fruits showed decay. The main mold was Botrytis cinerea. Ozone storage did not cause observable injury or defects. By 12 days, anthocyanin content of juice was similar to initial levels of all treatments. Surface color was better retained in 0.1 ppm-stored berries by 5 days and in 0.3 ppm-stored berries by 12 days, by hue angle values. Peroxidase was greater in controls and 0.1 ppm samples and was lowest in 0.3 ppm fruits by 12 days. Ozone storage resulted in market quality extension. Ozone has also been used in the control of post-harvest decay of table grapes caused by Rhizopus stolonifer (Sarig et al., 1996) Earlier studies have demonstrated that a novel source of ozone gas could be used to chemically degrade numerous mycotoxins, including aflatoxin (AF) B1. Subsequent in vitro analyses demonstrated detoxification of AFB1, suggesting a potential method of remediate AF-contaminated grain. McKenzie and co-workers (1998) investigated the ability of electrochemically produced ozone to degrade AFB1 in naturally contaminated whole kernel corn. Corn was procured from the southern coastal areas of Texas and HPLC analysis revealed 1,220 +/- 73.3 ppb AFB1. Control and contaminated corn were treated for 92 h with ozone at 200 mg/min in 30 kg batches; greater than 95% reduction of AFB1 in contaminated corn was achieved.
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The effects of gamma irradiation and ozone treatment on microbiological and physico-chemical properties of bee pollen were investigated (Yook et al., 1998). Gamma irradiation at 7.5 kGy reduced the total microbial loads below detection levels (>102 CFU/g), but after ozone treatment of upto 18 ppm for 8 h the total aerobic bacteria were found in concentrations of >103 CFU/g. Physico-chemical properties such as amino acid and fatty acid composition, thiobarbituric acid value, mineral content, and pigment were not significantly changed by gamma irradiation, whereas ozone treatment caused significant changes in fatty acid composition, thiobarbituric acid value and pigment by lipid oxidation and discoloration. E. Sanitation of poultry A pilot plant study of the effect of using an ozone contact system on the quality of poultry broiler carcasses and recirculating poultry chill water revealed lower carcass microbial levels and a destruction of all microbes (>99%) washed from the carcass in the chill water (Sheldon & Brown, 1986). Ozonation also reduced the chemical oxygen demand by a third and increased the light transmission of the treated chill water. The authors indicated that ozonation had no adverse effect on carcass color or lipid peroxidation, and did not produce a carcass off-flavor. Whistler and Sheldon (1989) evaluated ozone and formaldehyde as disinfectants in a prototype laboratory setter against microorganisms that are naturally present on fertile, freshly laid, broiler hatching eggs. Microbial counts were reduced by 2.5 log10 for water-misted and ozonated eggs or formaldehyde-fumigated eggs than for control and water-misted eggs. Eggshell conductance studies as measured by egg moisture losses in a desiccator showed no differences among the treatments. Hatchability was significantly reduced (26.5 to 37.5%) following ozonation (3.03% /wt for 2 h) in comparison with no treatment or water misting. Misting with ozonation was equally as effective as formaldehyde fumigation in reducing microbial counts. However, ozone treatment at the concentrations tested significantly reduced hatchability when compared with results of either no treatment, water misting, or an average hatchability figure for formaldehyde fumigation. These findings indicated that ozone is a good disinfectant yet may adversely affect embryo development when given in the gaseous form. Bailey and co-workers (1996) have conducted four trials to evaluate the efficacy of hatcher air sanitation utilizing ultraviolet light (UV), ozone, or hydrogen peroxide on bacterial populations, the spread of Salmonella, and hatchability of broiler eggs. The UV light (254 nm, 146 µ) and ozone (0.2 or 0.4 ppm) treatments were continuously applied through the final three days of hatch, the hydrogen peroxide treatment (2.5%) was administered 1 or 2 min of each 10 min at rates of 500 or 100 ml/h. Hatchability was not significantly reduced by sanitizing treatments when compared with the untreated control (94 versus 95.6%). As compared to controls, all sanitizing treatments reduced 75 to 99% of the total bacteria, Enterobacteriaceae, and Salmonella in the hatching cabinet air samples. The use of hydrogen peroxide resulted in greater reduction of bacteria than ozone or UV light. Only hydrogen peroxide significantly reduced Salmonella levels on eggshell fragments. Significant reductions in the number of Salmonella-positive chicks occurred using the ozone and hydrogen peroxide treatments. Hydrogen peroxide significantly reduced the magnitude of Salmonella colonization in chicken ceca. These trials demonstrated that the spread of bacteria could be effectively reduced in the hatching cabinet by air sanitation
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TABLE 2. Approved levels of ozone application Exposure
Ozone level (ppm)
Detectable odor OSHA 8 hr limit OSHA 1.5 min limit Lethal in few minutes
0.01 - 0.05 0.1 0.3 >1700
using UV light, ozone, and hydrogen peroxide. The potential to reduce bacterial cross contamination in the hatcher seems to be achievable without compromising the hatchability. F. Sanitation of sea-food Chen and co-workers (1992) have examined solubility and stability of ozone in shrimp-meat extract (SME), bactericidal effects on shrimp-meat organisms, mutagenicity of ozonated shrimp meat, and ozonolysis of DNA. The saturated concentration of ozone (1.4 ml/L) in SME was lower than in 2% saline or distilled water at 5 and 25˚C. Upon standing for 25 min after ozonation, ozone exhibited the same decomposition rate (2.7% /min) in SME at 5 and 25˚C. Among nine bacterial strains tested, Salmonella typhimurium was more resistant to ozone in shrimp meat. Mutagens were not detected in shrimp meat after ozonation in saline. Ozone in saline (