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Development of a Rep-PCR screening assay for enterotoxigenic Bacillus spp. in naturally contaminated food / Development of a repetitive element palindrome-polymerase chain reaction screening assay for enterotoxigenic Bacillus spp. in naturally contaminated food

Several powdered food products were screened using repetitive element palindrome PCR (rep-PCR) for the presence of enterotoxin producing species of Bacillus. Samples from these products were screened by being placed into a tryptone-peptoneglucose-yeast enrichment medium (TPGY), heat-treated, and shake-incubated. DNA was extracted using a modification of established protocol, leading to the development of an optimized method for each food system. Purified DNA was amplified through rep-PCR using extragenic sequence-targeting primers and optimized for each food product. Amplified PCR products were analyzed electrophoretically and viewed using an ultraviolet photodocumentation system. Bacillus cereus positive control DNA fingerprints were compared to banding patterns from enriched food samples, revealing the presence of the typical diagnostic 1,230 bp band in non-fat dry milk (NFDM). Restriction Fragment Length Polymorphism (RFLP) with Alu I restriction enzyme was performed on the 1230 bp diagnostic band from NFDM and displayed a profile consistent with Bacillus cereus positive control. RPLA (Reverse Passive Latex Agglutination) and BDE ELISA (Bacillus Diarrhoeal Enterotoxin Enzyme Linked Immunosorbent Assay - Tecra Diagnostics) confirmed the presence of HBL and NHE enterotoxin production in NFDM, Coffee creamer, infant milk formula, and two lecithin samples. / Department of Biology

Identiferoai:union.ndltd.org:BSU/oai:cardinalscholar.bsu.edu:handle/187726
Date January 2004
CreatorsCooper, Robin M.
ContributorsMcKillip, John L.
Source SetsBall State University
Detected LanguageEnglish
Formatviii, 29 leaves : ill. ; 28 cm.
SourceVirtual Press

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