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Development of a Melting-Curve-Based Multiplex Real-Time PCR Assay for the Simultaneous Detection of Viruses Causing Respiratory Infection.

Eliandro Reis TavaresThiago Ferreira de LimaGuilherme Bartolomeu-GonçalvesIsabela Madeira de CastroDaniel Gaiotto de LimaPaulo Henrique Guilherme BorgesGerson NakazatoRenata Katsuko Takayama KobayashiEmerson José VenancioCésar Ricardo Teixeira TarleyElaine Regina Delicato de AlmeidaMarsileni PelissonEliana Carolina VesperoAndrea Name Colado SimãoMárcia Regina Eches PeruginiGilselena KerbauyMarco Aurélio FornazieriMaria Cristina Bronharo TognimViviane Monteiro GóesTatiana de Arruda Campos Brasil de SouzaDanielle Bruna Leal OliveiraEdison Luiz DurigonLígia Carla Faccin-GalhardiLucy Megumi Yamauchi LioniSueli Fumie Yamada-Ogatta
Published in: Microorganisms (2023)
The prompt and accurate identification of the etiological agents of viral respiratory infections is a critical measure in mitigating outbreaks. In this study, we developed and clinically evaluated a novel melting-curve-based multiplex real-time PCR (M-m-qPCR) assay targeting the RNA-dependent RNA polymerase (RdRp) and nucleocapsid phosphoprotein N of SARS-CoV-2, the Matrix protein 2 of the Influenza A virus, the RdRp domain of the L protein from the Human Respiratory Syncytial Virus, and the polyprotein from Rhinovirus B genes. The analytical performance of the M-m-qPCR underwent assessment using in silico analysis and a panel of reference and clinical strains, encompassing viral, bacterial, and fungal pathogens, exhibiting 100% specificity. Moreover, the assay showed a detection limit of 10 copies per reaction for all targeted pathogens using the positive controls. To validate its applicability, the assay was further tested in simulated nasal fluid spiked with the viruses mentioned above, followed by validation on nasopharyngeal swabs collected from 811 individuals. Among them, 13.4% (109/811) tested positive for SARS-CoV-2, and 1.1% (9/811) tested positive for Influenza A. Notably, these results showed 100% concordance with those obtained using a commercial kit. Therefore, the M-m-qPCR exhibits great potential for the routine screening of these respiratory viral pathogens.
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