Real-time RT-PCR for the detection and quantitation of Oropouche virus
Share
Metadata
Show full item recordAuthor(s)
Rojas Segovia, Alejandra María; Stittleburg, Victoria; Cardozo Segovia, Fátima María; Bopp, Nathen; Cantero, César; López, Sanny; Bernal, Cynthia; Mendoza Torres, Laura Patricia; Aguilar, Patricia; Pinsky, Benjamin A.; Arévalo de Guillén, Yvalena; Páez Acchiardi, Gloria Malvina; Waggoner, Jesse J.Date of publishing
2019-09-09Type of publication
info:eu-repo/semantics/articleSubject(s)
Abstract
Oropouche virus (OROV) causes an acute, systemic febrile illness, and in certain regions of South America, this represents the second most common human arboviral infection after dengue virus. A new real-time RT-PCR was developed for OROV and reassortant species. The new OROV rRT-PCR proved linear across 6–7 orders of magnitude with a lower limit of 95% detection of 5.6–10.8 copies/μL. Upon testing dilutions of OROV and Iquitos virus reference genomic RNA, all dilutions with >10 copies/μL were detected in both the OROV rRT-PCR and a comparator molecular assay, but the OROV rRT-PCR detected more samples with ≤10 copies/μL (8/14 vs 0/13, respectively, P = 0.002). In a set of 100 acute-phase clinical samples from Paraguay patients with a suspected arboviral illness, no patients tested positive for OROV RNA using either assay. The OROV rRT-PCR provides a sensitive molecular assay for the study of this important yet neglected tropical arboviral infection.