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	Provedor de dados ArchiMer (17) Autor Hervio-heath, Dominique (17) Gourmelon, Michele (7) Catherine, Martial (4) Lozach, Solen (3) Monfort, Patrick (3) Colwell, Rita R. (2) Delesmont, R. (2) Esteves, Kevin (2) Jumas-bilak, Estelle (2) Mosser, Thomas (2) Tall, Amadou (2) Teillon, Anna (2) Touron-bodilis, A. (2) Amaro, Carmen (1) Andrieux-loyer, Francoise (1) Aujoulat, Fabien (1) Baker-austin, C. (1) Baker-austin, Craig (1) Baliere, Charlotte (1) Bayley, Amanda (1) Mais... Palavra-chave Coquillages (4) Bactéries pathogènes (3) Contamination microbiologique (3) Real-time PCR (3) Suivi (3) Vibrio (3) Microbial source tracking (2) Seafood (2) Shellfish (2) Water (2) Ancient DNA (1) Bactéries (1) Biochemical methods (1) Campylobacter (1) Coastal ecology (1) Coastal environment (1) Contamination (1) Conventional PCR (1) Culturable Vibrio spp (1) Dinoflagellates (1) Mais... Tipo do documento Text (17) Ano 2021 (1) 2019 (1) 2018 (1) 2017 (1) 2016 (2) 2015 (2) 2013 (2) 2012 (5) 2011 (1) 2010 (1) Mais... País France (17) Idioma Inglês (13) Francês (4)		Registro completo Provedor de dados:  ArchiMer País:  France Título:  Real-Time PCR optimization to identify environmental Vibrio spp. strains Autores:  Tall, Amadou Teillon, Anna Boisset, Claire Delesmont, R. Touron-bodilis, A. Hervio-heath, Dominique Data:  2012-08 Ano:  2012 Palavras-chave:  DnaJ Identification Real-time PCR Vibrio alginolyticus Vibrio cholerae Vibrio vulnificus Resumo:  Aims: To identify Vibrio vulnificus, Vibrio cholerae and Vibrio alginolyticus using standardized DNA extraction method and real-time PCR assays, among a large number of bacterial strains isolated from marine environment. Methods and Results: Methods for DNA extraction and real-time PCR were standardized to identify a large number of Vibrio spp. strains isolated through regular collection campaigns of environmental samples. Three real-time PCR assays were developed from a multiplex PCR, targeting V. vulnificus, V. cholerae and V. alginolyticus on the dnaJ gene. After testing their specificity, these systems were applied for the identification of 961 strains isolated at 22°C (446 strains) and 37°C (515 strains) in September 2009. The predominance of V. alginolyticus (82·6%) among the Vibrio spp. strains isolated at 37°C was shown. At 22°C, only 1·6% of the strains were identified by PCR and they were V. alginolyticus. Conclusions: Reproducible and specific real-time PCR assays combined to a DNA extraction method on microplates were used to constitute a large environmental Vibrio strains collection and to identify and detect potential human pathogenic Vibrio isolated at 37°C. For environmental strains isolated at 22°C, because of the higher species diversity, other approaches, like sequencing, should be chosen for identification. Significance and Impact of the Study: The protocol developed in this study provides an appropriate and rapid screening tool to identify a large number of bacterial strains routinely isolated from the environment in long-term studies. Tipo:  Text Idioma:  Inglês Identificador:  http://archimer.ifremer.fr/doc/00088/19901/17562.pdf DOI:10.1111/j.1365-2672.2012.05350.x Editor:  Wiley-blackwell Relação:  http://archimer.ifremer.fr/doc/00088/19901/ Formato:  application/pdf Fonte:  Journal Of Applied Microbiology (1364-5072) (Wiley-blackwell), 2012-08 , Vol. 113 , N. 2 , P. 361-372 Direitos:  2012 The Authors Journal of Applied Microbiology © 2012 The Society for Applied Microbiology Fechar

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