Validation of use of the miniPCR thermocycler for Ebola and Zika virus detection

dc.contributor.affiliationInstituto Tecnológico y de Estudios Superiores de Monterreyes_MX
dc.contributor.authorGonzález González, Everardo
dc.contributor.authorMendoza Ramos, Jackelin Lizeth
dc.contributor.authorPedroza, Sara Cristina
dc.contributor.authorCuellar Monterrubio, Aimé Alexandra
dc.contributor.authorMárquez Ipiña, Alan Roberto
dc.contributor.authorLira Serhan, Daniel
dc.contributor.authorTrujillo de Santiago, Grissel
dc.contributor.authorMoisés Alvarez, Mario
dc.date.accessioned2022-06-29T22:27:40Z
dc.date.available2022-06-29T22:27:40Z
dc.date.issued2019-05-09
dc.description.abstractThe development of point-of-care (POC) diagnostic systems has received well-deserved attention in recent years in the scientific literature, and many experimental systems show great promise in real settings. However, in the case of an epidemic emergency (or a natural disaster), the first line of response should be based on commercially available and validated resources. Here, we compare the performance and ease of use of the miniPCR, a recently commercially available compact and portable PCR device, and a conventional thermocycler for the diagnostics of viral nucleic acids. We used both thermocyclers to detect and amplify Ebola and Zika DNA sequences of different lengths (in the range of 91 to 300 nucleotides) at different concentrations (in the range of ~50 to 4.0 x 108 DNA copies). Our results suggest that the performance of both thermocyclers is quite similar. Moreover, the portability, ease of use, and reproducibility of the miniPCR makes it a reliable alternative for point-of-care nucleic acid detection and amplification.es_MX
dc.format.mediumTextoes_MX
dc.identificator3||32||2302||230221es_MX
dc.identifier.citationGonzález-González E, Mendoza-Ramos JL, Pedroza SC, Cuellar-Monterrubio AA, Márquez-Ipiña AR, Lira-Serhan D, et al. (2019) Validation of use of the miniPCR thermocycler for Ebola and Zika virus detection. PLoS ONE 14(5): e0215642. https://doi.org/10.1371/journal.pone.0215642es_MX
dc.identifier.doihttps://doi.org/10.1371/journal.pone.0215642
dc.identifier.issue5es_MX
dc.identifier.journalPLoS ONEes_MX
dc.identifier.urihttps://hdl.handle.net/11285/648506
dc.identifier.volume14es_MX
dc.language.isoenges_MX
dc.relation.isFormatOfpublishedVersiones_MX
dc.relation.urlhttps://journals.plos.org/plosone/article?id=10.1371/journal.pone.0215642es_MX
dc.rightsopenAccesses_MX
dc.rights.urihttp://creativecommons.org/licenses/by/4.0es_MX
dc.subjectMEDICINA Y CIENCIAS DE LA SALUD::CIENCIAS MÉDICAS::BIOQUÍMICA::BIOLOGÍA MOLECULARes_MX
dc.subject.countryEstados Unidos de América / United Stateses_MX
dc.subject.keywordPolymerase chain reactiones_MX
dc.subject.keywordEbola viruses_MX
dc.subject.keywordZika viruses_MX
dc.subject.keywordAgarose gel electrophoresises_MX
dc.subject.keywordNucleic acidses_MX
dc.subject.keywordGel electrophoresises_MX
dc.subject.keywordViral packaginges_MX
dc.subject.keywordViral nucleic acides_MX
dc.subject.lcshTechnologyes_MX
dc.titleValidation of use of the miniPCR thermocycler for Ebola and Zika virus detectiones_MX
dc.typeArtículo

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