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dc.contributor.authorAuthorLuraschi, Roberto
dc.contributor.authorAuthorSantibáñez, Álvaro
dc.contributor.authorAuthorBarrera-Avalos, Carlos.
dc.contributor.authorAuthorVallejos-Vidal, Eva
dc.contributor.authorAuthorMateluna-Flores, Carlos.
dc.contributor.authorAuthorAlarcón, Javiera
dc.contributor.authorAuthorCayunao, Javiera
dc.contributor.authorAuthorMella-Torres, Andrea.
dc.contributor.authorAuthorHernández, Felipe
dc.contributor.authorAuthorInostroza-Molina, Ailen.
dc.contributor.authorAuthorValdés, Daniel
dc.contributor.authorAuthorImarai, Mónica
dc.contributor.authorAuthorAcuña-Castillo, Claudio.
dc.contributor.authorAuthorReyes-López, Felipe E.
dc.contributor.authorAuthorSandino, Ana María
dc.date.accessionedDate Accessioned2024-09-03T19:19:13Z
dc.date.availableDate Available2024-09-03T19:19:13Z
dc.date.issuedDate Issued2022
dc.identifier.citationReferencia BibliográficaFrontiers in Public Health, 10, 15 p.
dc.identifier.issnISSN2296-2565
dc.identifier.uriURIhttp://repositorio.udla.cl/xmlui/handle/udla/1434
dc.identifier.uriURIhttps://www.frontiersin.org/journals/public-health
dc.description.abstractAbstractIntroduction: The COVID-19 pandemic is still in force, causing global public health challenges and threats. Although vaccination and herd immunity have proven to be the most efficient way to control the pandemic, massive and early testing of patients using the RT-qPCR technique is crucial for constant genomic surveillance. The appearance of variants of SARS-CoV-2 with new mutations can reduce the efficiency of diagnostic detection. In this sense, several commercial RT-qPCR kits have been the target of extensive analysis because low assay performance could lead to false-negative diagnoses. Methods: In this study, we evaluated the performance of three commercial RT-qPCR kits; Thermo Fisher (TaqMan 2019-nCoV Assay Kit v1), BGI and Roche (LightCycler® Multiplex RNA Virus Master) used for the diagnosis of COVID-19 throughout the pandemic in Santiago de Chile. Results: Under our best assay conditions, we found significant differences in Cq amplification values for control and viral probes, against the same nasopharyngeal swab samples (NPSs). In addition, in some cases, the sensitivity of the RT-qPCR kits decreased against viral variants. Conclusion: Our study suggests evaluating the RT-qPCR kits used to detect SARS-CoV-2 because variants such as Omicron, which has several mutations, can compromise their detection and underestimate viral circulation.
dc.format.extentdc.format.extent15 páginas
dc.format.extentdc.format.extent8.547Mb
dc.format.mimetypedc.format.mimetypePDF
dc.language.isoLanguage ISOeng
dc.publisherPublisherFrontiers Media
dc.rightsRightsCreative Commons Attribution License (CC BY)
dc.sourceSourcesFrontiers in Public Health
dc.subjectSubjectDiagnostic sensitivity
dc.subjectSubjectGenomic surveillance
dc.subjectSubjectRT-qPCR
dc.subject.lcshdc.subject.lcshCOVID-19 (Enfermedad)
dc.titleTitleEvaluation and comparison of the sensitivity of three commercial RT-qPCR kits used for the detection of SARS-CoV-2 in Santiago, Chile
dc.typeDocument TypeArtículo
dc.udla.catalogadordc.udla.catalogadorCBM
dc.udla.indexdc.udla.indexScience Citation Index Expanded
dc.udla.indexdc.udla.indexScopus
dc.udla.indexdc.udla.indexSocial Sciences Citation Index
dc.udla.indexdc.udla.indexDOAJ
dc.udla.indexdc.udla.indexEMBASE
dc.udla.indexdc.udla.indexMEDLINE
dc.udla.indexdc.udla.indexPsycinfo
dc.identifier.doidc.identifier.doi10.3389/fpubh.2022.1010336
dc.facultaddc.facultadFacultad de Medicina Veterinaria y Agronomía


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