Quantitation and application of bacteriocins in food

Quantitation and application of bacteriocins in food

Several obstacles to widespread use of bacteriocins in food have been identified, including lack of specific, rapid quantitation methods, and little data on their efficacy in food systems. The first objective of this study was to develop a specific, rapid quantitation method for bacteriocins that d...

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Bibliographic Details
Main Author: Haveroen, Melissa E
Other Authors: McMullen, Lynn (Department of Agricultural, Food and Nutritional Science)
Format: Others
Language:en
Published: 2011
Subjects:
bacteriocin
food safety
Clostridium botulinum
lactic acid bacteria
brochocin-C
antibody
quantitation
Online Access:http://hdl.handle.net/10048/1882
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spelling ndltd-LACETR-oai-collectionscanada.gc.ca-AEU.10048-18822012-03-21T22:50:08ZMcMullen, Lynn (Department of Agricultural, Food and Nutritional Science)Bressler, David (Department of Agricultural, Food and Nutritional Science)Haveroen, Melissa E2011-04-13T16:29:29Z2011-04-13T16:29:29Z2011-04-13T16:29:29Zhttp://hdl.handle.net/10048/1882Several obstacles to widespread use of bacteriocins in food have been identified, including lack of specific, rapid quantitation methods, and little data on their efficacy in food systems. The first objective of this study was to develop a specific, rapid quantitation method for bacteriocins that did not rely on bioassays and their associated limitations. Phage display was chosen to reduce reliance on continued use of animals and produce antibodies to the bacteriocins leucocin A, piscicolin 126, and brochocin-A. Although the antibody libraries generated by phage display were not successful for antibody production, a strong immune response to leucocin A and piscicolin 126 was observed in mice. The second objective of the study was to determine the efficacy of brochocin-C against Clostridium botulinum in a model system and in a vacuum-packaged, chopped and formed pork product stored at refrigeration temperature. Group I Cl. botulinum was not controlled by brochocin-C, and was found to inactivate brochocin-C and several class IIa bacteriocins by proteolysis. Cell counts revealed that Group II Cl. botulinum was controlled by brochocin-C in a model meat system, but was not controlled in the chopped and formed pork product. Powdered smoke and NaCl in the pork product had a synergistic interaction against Group II Cl. botulinum, as shown by minimum inhibitory concentration testing. The choice of media for isolation of Cl. botulinum from the chopped and formed pork product was important, as the presence of background microflora isolated from the meat was found to impact growth of Group II Cl. botulinum on plating media. In the presence of the background microflora, which were identified by 16S rDNA sequencing as carnobacteria and staphylococci, inclusion of phosphate in the plating medium was found to allow growth of Cl. botulinum. Other nutrients such as magnesium, sulphur, or increased protein sources added to the medium had no effect on growth of Cl. botulinum. Two of the background microflora strains, Carnobacterium maltaromaticum MH3 and Staphylococcus pasteuri EIV-21, inhibited Cl. botulinum, while one strain, C. maltaromaticum MH2, stimulated growth of Cl. botulinum.1689755 bytesapplication/pdfenbacteriocinfood safetyClostridium botulinumlactic acid bacteriabrochocin-CantibodyquantitationQuantitation and application of bacteriocins in foodThesisDoctor of PhilosophyDoctoralDepartment of Agricultural, Food and Nutritional ScienceUniversity of Alberta2011-06Food Science and TechnologyGänzle, Michael (Department of Agricultural, Food and Nutritional Science)Vederas, John (Department of Chemistry)Worobo, Randy (Department of Food Science, Cornell University)
collection NDLTD
language en
format Others
sources NDLTD
topic bacteriocin
food safety
Clostridium botulinum
lactic acid bacteria
brochocin-C
antibody
quantitation
spellingShingle bacteriocin
food safety
Clostridium botulinum
lactic acid bacteria
brochocin-C
antibody
quantitation
Haveroen, Melissa E
Quantitation and application of bacteriocins in food
description Several obstacles to widespread use of bacteriocins in food have been identified, including lack of specific, rapid quantitation methods, and little data on their efficacy in food systems. The first objective of this study was to develop a specific, rapid quantitation method for bacteriocins that did not rely on bioassays and their associated limitations. Phage display was chosen to reduce reliance on continued use of animals and produce antibodies to the bacteriocins leucocin A, piscicolin 126, and brochocin-A. Although the antibody libraries generated by phage display were not successful for antibody production, a strong immune response to leucocin A and piscicolin 126 was observed in mice. The second objective of the study was to determine the efficacy of brochocin-C against Clostridium botulinum in a model system and in a vacuum-packaged, chopped and formed pork product stored at refrigeration temperature. Group I Cl. botulinum was not controlled by brochocin-C, and was found to inactivate brochocin-C and several class IIa bacteriocins by proteolysis. Cell counts revealed that Group II Cl. botulinum was controlled by brochocin-C in a model meat system, but was not controlled in the chopped and formed pork product. Powdered smoke and NaCl in the pork product had a synergistic interaction against Group II Cl. botulinum, as shown by minimum inhibitory concentration testing. The choice of media for isolation of Cl. botulinum from the chopped and formed pork product was important, as the presence of background microflora isolated from the meat was found to impact growth of Group II Cl. botulinum on plating media. In the presence of the background microflora, which were identified by 16S rDNA sequencing as carnobacteria and staphylococci, inclusion of phosphate in the plating medium was found to allow growth of Cl. botulinum. Other nutrients such as magnesium, sulphur, or increased protein sources added to the medium had no effect on growth of Cl. botulinum. Two of the background microflora strains, Carnobacterium maltaromaticum MH3 and Staphylococcus pasteuri EIV-21, inhibited Cl. botulinum, while one strain, C. maltaromaticum MH2, stimulated growth of Cl. botulinum. === Food Science and Technology
author2 McMullen, Lynn (Department of Agricultural, Food and Nutritional Science)
author_facet McMullen, Lynn (Department of Agricultural, Food and Nutritional Science)
Haveroen, Melissa E
author Haveroen, Melissa E
author_sort Haveroen, Melissa E
title Quantitation and application of bacteriocins in food
title_short Quantitation and application of bacteriocins in food
title_full Quantitation and application of bacteriocins in food
title_fullStr Quantitation and application of bacteriocins in food
title_full_unstemmed Quantitation and application of bacteriocins in food
title_sort quantitation and application of bacteriocins in food
publishDate 2011
url http://hdl.handle.net/10048/1882
work_keys_str_mv AT haveroenmelissae quantitationandapplicationofbacteriocinsinfood
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