Molecular diagnosis of dengue

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dc.contributor(LEDM) Lab. Estratégico de Diagnóstico Molecularpt_BR
dc.contributor.authorNunes, Priscila C. G.pt_BR
dc.contributor.authorLima, Monique da Rocha Queirozpt_BR
dc.contributor.authorSantos, Flávia B. dospt_BR
dc.date.accessioned2022-02-18T18:52:47Z-
dc.date.available2022-02-18T18:52:47Z-
dc.date.issued2021pt_BR
dc.identifier.isbn978-1-0716-1878-3pt_BR
dc.identifier.urihttps://repositorio.butantan.gov.br/handle/butantan/4209-
dc.description.abstractSeveral protocols for genomic amplification using reverse transcription followed by polymerase chain reaction (RT-PCR), important in the identification of the infecting serotype, have been used in the rapid diagnosis of Dengue Virus (DENV) infections. The qualitative protocol described by Lanciotti et al. (J Clin Microbiol 30: 545–551, 1992) suggested by WHO detects the four DENV serotypes simultaneously in one procedure “semi-nested,” generating amplified products with specific sizes in base pairs for each serotype and it has been the most used in the past two decades. However, advances in molecular diagnosis have enabled the development of RT-PCR in real time (qRT-PCR) based on the use of dyes and probes (SYBR green and TaqMan), which is performed in a single step and is capable of providing quantitative data. In addition to quantification, the advantages of qRT-PCR over conventional RT-PCR include speed, greater sensitivity and specificity, and low rate of false positives. Several protocols for the diagnosis and/or quantification of DENV have already been described. Non-PCR-based methods such as reverse transcription loop-mediated isothermal amplification have shown high sensitivities and specificities. RT-PCR and qRT-PCR techniques can be performed using serum, plasma, infected cells, mosquitoes, fresh, and paraffin-embedded tissues. However, despite fast and accurate, they are limited to samples collected during the acute phase of infection (up to 7 days after the onset of symptoms) and require specialized equipment and trained staff.pt_BR
dc.format.extent15 p.pt_BR
dc.language.isoEnglishpt_BR
dc.publisherHumanapt_BR
dc.relation.ispartofseries2409pt_BR
dc.rightsRestricted accesspt_BR
dc.titleMolecular diagnosis of denguept_BR
dc.typeBook chapterpt_BR
dc.identifier.doi10.1007/978-1-0716-1879-0_11pt_BR
dc.contributor.external(IOC) Instituto Oswaldo Cruzpt_BR
dc.contributor.external(FIOCRUZ) Fundação Oswaldo Cruzpt_BR
dc.contributor.external(SIEVS/RJ) Superintendência de Informações Estratégicas de Vigilância em Saúde do Rio de Janeiropt_BR
dc.contributor.external(LASP) Laboratório Municipal de Saúde Públicapt_BR
dc.publisher.cityNew Yorkpt_BR
dc.subject.keywordMolecular diagnosispt_BR
dc.subject.keywordRT-PCRpt_BR
dc.subject.keywordqRT-PCRpt_BR
dc.subject.keywordSYBR greenpt_BR
dc.subject.keywordTaqManpt_BR
dc.identifier.citationabntv. 2409, p. 157-171, out. 2021pt_BR
dc.identifier.citationvancouver2021 Oct; 2409: 157-171pt_BR
dc.publisher.countryUnited Statespt_BR
dc.contributor.butantanLima, Monique da Rocha Queiroz|:Tecnologista|:(LEDM) Lab. Estratégico de Diagnóstico Molecularpt_BR
dc.identifier.bvsccBR78.1pt_BR
dc.identifier.bvsdbIBProdpt_BR
dc.relation.ispartofbookMethods in Molecular Biologypt_BR
dc.contributor.externalcountryBrazilpt_BR
dc.description.dbindexedYespt_BR
item.fulltextSem Texto completo-
item.openairetypeBook chapter-
item.languageiso639-1English-
item.grantfulltextnone-
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