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dc.contributor.authorDillon, Davin C.-
dc.contributor.authorAlderson, Mark R.-
dc.contributor.authorDay, Craig H.-
dc.contributor.authorBement, Teresa-
dc.contributor.authorCampos Neto, Antonio-
dc.contributor.authorSkeiky, Yasir A. W.-
dc.contributor.authorVedvick, Thomas S.-
dc.contributor.authorBadaró, Roberto José da Silva-
dc.contributor.authorReed, Steven G.-
dc.contributor.authorHoughton, Raymond-
dc.creatorDillon, Davin C.-
dc.creatorAlderson, Mark R.-
dc.creatorDay, Craig H.-
dc.creatorBement, Teresa-
dc.creatorCampos Neto, Antonio-
dc.creatorSkeiky, Yasir A. W.-
dc.creatorVedvick, Thomas S.-
dc.creatorBadaró, Roberto José da Silva-
dc.creatorReed, Steven G.-
dc.creatorHoughton, Raymond-
dc.date.accessioned2012-12-03T19:33:32Z-
dc.date.issued2000-09-
dc.identifier.issn0095-1137-
dc.identifier.urihttp://www.repositorio.ufba.br/ri/handle/ri/7307-
dc.descriptionp.3285–3290pt_BR
dc.description.abstractIn order to identify antigens that may be used in the serodiagnosis of active tuberculosis (TB), we screened a Mycobacterium tuberculosis genomic expression library with a pool of sera from patients diagnosed with active pulmonary TB. The sera used lacked reactivity with a recombinant form of the M. tuberculosis 38-kDa antigen (r38kDa), and the goal was to identify antigens that might complement r38kDa in a serodiagnostic assay. Utilizing this strategy, we identified a gene, previously designated lhp, which encodes a 100-amino-acid protein referred to as culture filtrate protein 10 (CFP-10). The lhp gene is located directly upstream of esat-6, within a region missing in M. bovis BCG. Immunoblot analysis demonstrated that CFP-10 is present in M. tuberculosis CFP, indicating that it is likely a secreted or shed antigen. Purified recombinant CFP-10 (rCFP-10) was shown to be capable of detecting specific antibody in a percentage of TB patients that lack reactivity with r38kDa, most notably in smear-negative cases, where sensitivity was increased from 21% for r38kDa alone to 40% with the inclusion of rCFP-10. In smear-positive patient sera, sensitivity was increased from 49% for r38kDa alone to 58% with the inclusion of rCFP-10. In addition, rCFP-10 was shown to be a potent T-cell antigen, eliciting proliferative responses and gamma interferon production from peripheral blood mononuclear cells in 70% of purified protein derivative-positive individuals without evident disease. The responses to this antigen argue for the inclusion of rCFP-10 in a polyvalent serodiagnostic test for detection of active TB infection. rCFP-10 could also contribute to the development of a recombinant T-cell diagnostic test capable of detecting exposure to M. tuberculosis.pt_BR
dc.language.isoenpt_BR
dc.titleMolecular and immunological characterization of mycobacterium tuberculosis CFP-10, an immunodiagnostic antigen missing in mycobacterium bovis BCGpt_BR
dc.title.alternativeJournal of Clinical Mircobiologypt_BR
dc.typeArtigo de Periódicopt_BR
dc.identifier.numberv. 38, n. 9pt_BR
dc.embargo.liftdate10000-01-01-
Aparece nas coleções:Artigo Publicado em Periódico (Faculdade de Medicina)

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