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Rapid detection of Mycobacterium tuberculosis DNA and genetic markers for Isoniazid resistance in Ziehl-Neelsen stained slides.

Use este link compartilhar ou citar este material: http://educapes.capes.gov.br/handle/capes/1003085
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Autor(es): dc.creatorBello, Graziele Lima-
Autor(es): dc.creatorMorais, Franciele Costa Leite-
Autor(es): dc.creatorJesus, Sheile Pinheiro de-
Autor(es): dc.creatorWolf, Jonas Michel-
Autor(es): dc.creatorGehlen, Mirela-
Autor(es): dc.creatorAlmeida, Isabela Neves de-
Autor(es): dc.creatorFigueredo, Lida Jouca de Assis-
Autor(es): dc.creatorSoares, Tainá dos Santos-
Autor(es): dc.creatorBarcellos, Regina Bones-
Autor(es): dc.creatorCosta, Elis Regina Dalla-
Autor(es): dc.creatorMiranda, Silvana Spíndola de-
Autor(es): dc.creatorRossetti, Maria Lucia Rosa-
Data de aceite: dc.date.accessioned2025-08-21T15:07:48Z-
Data de disponibilização: dc.date.available2025-08-21T15:07:48Z-
Data de envio: dc.date.issued2023-01-15-
Data de envio: dc.date.issued2023-01-15-
Data de envio: dc.date.issued2019-
Fonte completa do material: dc.identifierhttp://www.repositorio.ufop.br/jspui/handle/123456789/15948-
Fonte completa do material: dc.identifierhttps://doi.org/10.1590/0074-02760190407-
Fonte: dc.identifier.urihttp://educapes.capes.gov.br/handle/capes/1003085-
Descrição: dc.descriptionBACKGROUND Early diagnosis of tuberculosis (TB) and identification of strains of Mycobacterium tuberculosis resistant to anti- TB drugs are considered the main factors for disease control. OBJECTIVES To standardise a real-time polymerase chain reaction (qPCR) assay technique and apply it to identify mutations involved in M. tuberculosis resistance to Isoniazid (INH) directly in Ziehl-Neelsen (ZN) stained slides. METHODS Were analysed 55 independent DNA samples extracted from clinical isolates of M. tuberculosis by sequencing. For application in TB diagnosis resistance, 59 ZN-stained slides were used. The sensitivity, specificity and Kappa index, with a 95% confidence interval (CI95%), were determined. FINDINGS The agreement between the tests was, for the katG target, the Kappa index of 0.89 (CI95%: 0.7-1.0). The sensitivity and specificity were 97.6% (CI95%: 87.7-99.9) and 91.7% (CI95%: 61.5-99.5), respectively. For inhA, the Kappa index was 0.92 (CI95%: 0.8-1.0), the sensitivity and specificity were 94.4% (CI95%: 72.7-99.8) and 97.3% (CI95%: 85.8-99.9), respectively. The use of ZN- stained slides for drug-resistant TB detection showed significant results when compared to other standard tests for drug resistance. MAIN CONCLUSIONS qPCR genotyping proved to be an efficient method to detect genes that confer M. tuberculosis resistance to INH. Thus, qPCR genotyping may be an alternative instead of sequencing.-
Formato: dc.formatapplication/pdf-
Idioma: dc.languageen-
Direitos: dc.rightsaberto-
Direitos: dc.rightsThis is an open access article distributed under the terms of the Creative Commons license. Fonte: o PDF do artigo.-
Palavras-chave: dc.subjectGenotyping-
Palavras-chave: dc.subjectReal-time PCR-
Título: dc.titleRapid detection of Mycobacterium tuberculosis DNA and genetic markers for Isoniazid resistance in Ziehl-Neelsen stained slides.-
Aparece nas coleções:Repositório Institucional - UFOP

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