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Detection of the mecA gene and identification of Staphylococcus directly from blood culture bottles by multiplex polymerase chain reaction

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dc.contributor.authorRocchetti, Taisa Trevizani [UNESP]
dc.contributor.authorMartins, Katheryne Benini [UNESP]
dc.contributor.authorMartins, Patricia Yoshida Faccioli [UNESP]
dc.contributor.authorOliveira, Rogério Antonio de [UNESP]
dc.contributor.authorMondelli, Alessandro Lia [UNESP]
dc.contributor.authorFortaleza, Carlos Magno Castelo Branco [UNESP]
dc.contributor.authorCunha, Maria de Lourdes Ribeiro de Souza da [UNESP]
dc.contributor.institutionUniversidade Estadual Paulista (Unesp)
dc.date.accessioned2018-12-11T17:19:37Z
dc.date.available2018-12-11T17:19:37Z
dc.date.issued2018-03-01
dc.description.abstractIntroduction: Staphylococcus spp. – both S. aureus, including methicillin-resistant strains (MRSA) and coagulase negative staphylococci (CoNS) – are relevant agents of healthcare-associated infections. Therefore, the rapid recognition of MRSA and methicillin-resistant CoNS from blood stream infections is critically important for patient management. It is worth noting that inappropriate empiric therapy has been associated with higher in-hospital mortality. Material and methods: In this study we evaluated a multiplex polymerase chain reaction (multiplex PCR) standardized to detect Staphylococcus spp., S. aureus, and mecA gene-encoded oxacillin resistance directly from blood culture bottles. A total of 371 blood cultures with Gram-positive microorganisms confirmed by Gram-stain were analyzed. Results from multiplex PCR were compared to phenotypic characterization of isolates. Results: Staphylococcus aureus was detected in 85 (23.0%) blood cultures and CoNS in 286 (77.0%). There was 100% agreement between phenotypic and multiplex PCR identification. Forty-three (50.6%) of the 85 S. aureus carried the mecA gene and among the 286 CoNS, 225 (78.7%) were positive for the mecA gene. Conclusions: The multiplex PCR assay developed here was found to be sensitive, specific, rapid, and showed good agreement with the phenotypic results besides being less expensive. This PCR method could be used in clinical laboratories for rapid identification and initiation of specific and effective treatment, reducing patient mortality and morbidity. Furthermore, this method may reduce misuse of antimicrobial classes that are more expensive and toxic, thus contributing to the selection of antibiotic-resistant Staphylococcus spp.en
dc.description.affiliationUNESP - Univ Estadual Paulista Instituto de Biociências de Botucatu Departamento de Microbiologia e Imunologia
dc.description.affiliationUNESP - Univ Estadual Paulista Faculdade de Medicina de Botucatu Hospital Universitário Departamento de Doenças Tropicais
dc.description.affiliationUNESP - Univ Estadual Paulista Instituto de Biociências de Botucatu Departamento de Biociência
dc.description.affiliationUNESP - Univ Estadual Paulista Faculdade de Medicina de Botucatu Hospital Universitário Departamento de Medicina Interna
dc.description.affiliationUnespUNESP - Univ Estadual Paulista Instituto de Biociências de Botucatu Departamento de Microbiologia e Imunologia
dc.description.affiliationUnespUNESP - Univ Estadual Paulista Faculdade de Medicina de Botucatu Hospital Universitário Departamento de Doenças Tropicais
dc.description.affiliationUnespUNESP - Univ Estadual Paulista Instituto de Biociências de Botucatu Departamento de Biociência
dc.description.affiliationUnespUNESP - Univ Estadual Paulista Faculdade de Medicina de Botucatu Hospital Universitário Departamento de Medicina Interna
dc.description.sponsorshipConselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq)
dc.description.sponsorshipFundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)
dc.description.sponsorshipIdFAPESP: 2010/14250-0
dc.format.extent99-105
dc.identifierhttp://dx.doi.org/10.1016/j.bjid.2018.02.006
dc.identifier.citationBrazilian Journal of Infectious Diseases, v. 22, n. 2, p. 99-105, 2018.
dc.identifier.doi10.1016/j.bjid.2018.02.006
dc.identifier.file2-s2.0-85045855237.pdf
dc.identifier.issn1678-4391
dc.identifier.issn1413-8670
dc.identifier.lattes0115647772315973
dc.identifier.scopus2-s2.0-85045855237
dc.identifier.urihttp://hdl.handle.net/11449/176214
dc.language.isoeng
dc.relation.ispartofBrazilian Journal of Infectious Diseases
dc.relation.ispartofsjr0,817
dc.rights.accessRightsAcesso abertopt
dc.sourceScopus
dc.subjectBlood cultures
dc.subjectmecA gene
dc.subjectMRSA
dc.subjectMultiplex PCR
dc.subjectStaphylococcus aureus
dc.subjectStaphylococcus spp.
dc.titleDetection of the mecA gene and identification of Staphylococcus directly from blood culture bottles by multiplex polymerase chain reactionen
dc.typeArtigopt
dspace.entity.typePublication
relation.isOrgUnitOfPublicationa3cdb24b-db92-40d9-b3af-2eacecf9f2ba
relation.isOrgUnitOfPublicationab63624f-c491-4ac7-bd2c-767f17ac838d
relation.isOrgUnitOfPublication.latestForDiscoverya3cdb24b-db92-40d9-b3af-2eacecf9f2ba
unesp.author.lattes7697507273984482[5]
unesp.author.lattes0115647772315973
unesp.author.lattes2589937673452910[6]
unesp.author.orcid0000-0002-4401-5656[5]
unesp.author.orcid0000-0003-4120-1258[6]
unesp.campusUniversidade Estadual Paulista (UNESP), Faculdade de Medicina, Botucatupt
unesp.campusUniversidade Estadual Paulista (UNESP), Instituto de Biociências, Botucatupt
unesp.departmentDoenças Tropicais e Diagnósticos por Imagem - FMBpt
unesp.departmentMicrobiologia e Imunologia - IBBpt

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Botucatu - IBB - Instituto de Biociências
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