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Use este identificador para citar ou linkar para este item: https://repositorio.ufba.br/handle/ri/7875
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dc.contributor.authorAlmeida, Paulo Fernando de-
dc.contributor.authorAlmeida, Rogeria Comastri de Castro-
dc.creatorAlmeida, Paulo Fernando de-
dc.creatorAlmeida, Rogeria Comastri de Castro-
dc.date.accessioned2013-01-16T11:36:34Z-
dc.date.issued2000-
dc.identifier.issn0956-7135-
dc.identifier.urihttp://www.repositorio.ufba.br/ri/handle/ri/7875-
dc.descriptionTexto completo: acesso restrito. p. 97–101pt_BR
dc.description.abstractPolymerase chain reaction is a powerful technique for detection of pathogens in foods. It is a rapid procedure with both sensitivity and specificity for quick detection and identification of specific pathogenic bacteria from different sources. Listeria monocytogenes detection methods based on PCR amplification of the iap, prfA and hly gene sequences have been reported. The present study undertakes the development of an alternative PCR method using the inl gene sequences as a target to detect pathogenic L. monocytogenes. The presence of a unique and specific DNA amplification fragment of 760 bp for the intragenic repeats B of the inlA gene in all strains of L. monocytogenes as compared to none in other Listeria and unrelated Gram positive and Gram negative species confirms that this procedure is an alternative PCR protocol for detection of L. monocytogenes.pt_BR
dc.language.isoenpt_BR
dc.sourcehttp://dx.doi.org/10.1016/S0956-7135(99)00067-5pt_BR
dc.subjectPCRpt_BR
dc.subjectListeria monocytogenespt_BR
dc.subjectInternalinpt_BR
dc.titleA PCR protocol using inl gene as a target for specific detection of Listeria monocytogenespt_BR
dc.title.alternativeFood Controlpt_BR
dc.typeArtigo de Periódicopt_BR
dc.identifier.numberv. 11, n. 2pt_BR
dc.embargo.liftdate10000-01-01-
Aparece nas coleções:Artigo Publicado em Periódico (ICS)

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