Detection of Listeria monocytogenes in food using a combined enrichment/real-time PCR method targeting the prfA gene |
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Authors: | Rossmanith Peter Krassnig Martina Wagner Martin Hein Ingeborg |
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Affiliation: | 1. Environment and Biotechnology Centre, Faculty of Life and Social Sciences, Swinburne University of Technology, PO Box 218, Hawthorn 3122 Victoria, Australia;2. bioMérieux Australia Pty Ltd, Unit 25 Parkview Business Centre, 1 Maitland Place, Baulkham Hills, NSW 2153, Australia;1. Subdirección de Investigación y Tecnología, Instituto Tecnológico Agrario de Castilla y León (ITACyL), Carretera de Burgos Km, 119, Valladolid, Spain;2. Microbiology Section, Faculty of Sciences, University of Burgos, Plaza Misael Bauñuelos s/n, 9001 Burgos, Spain;3. Istituto Superiore di Sanità, Veterinary Public Health and Food Safety Department, Viale Regina Elena 299, 00161 Rome, Italy |
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Abstract: | A combined enrichment/real-time PCR method for the detection of Listeria monocytogenes is presented. The method is based on a conventional PCR assay targeting the prfA gene, which has been validated and suggested as an international standard PCR method for identifying L. monocytogenes in food. This real-time PCR assay includes an internal amplification control. Inclusivity and exclusivity were 100% each when testing 100 L. monocytogenes isolates, 30 Listeria spp. isolates other than L. monocytogenes, and 29 non-Listeria isolates. The theoretical detection limit was one copy of the target gene per PCR reaction and the practical detection limit was about 5 copies per PCR. Using the combined enrichment/real-time PCR method, 7.5 CFU/25 ml of artificially contaminated raw milk, and 9, 1, and 1 CFU/15 g of artificially contaminated salmon, paté, and green-veined cheese, respectively, were detected. When analyzing 76 naturally contaminated food samples of various types and comparing the results with the ISO 11290-1 standard method, the relative accuracy was 96%, the relative specificity 100%, and the relative sensitivity, 76.9%. |
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