| Literature DB >> 20116400 |
Maria Luisa Carrozza1, Maurizio Mazzei, Patrizia Bandecchi, Christophe Fraisier, Marta Pérez, Marie Suzan-Monti, Damian de Andrés, Beatriz Amorena, Sergio Rosati, Valgerdur Andrésdottir, Lluis Lujan, Michel Pepin, Barbara Blacklaws, Francesco Tolari, Gordon D Harkiss.
Abstract
The aim of this study was the development of gag and pol dual labelled probe real-time PCR and RT PCR assays to quantify the proviral load and the transcripts of the British Visna/maedi virus EV1 strain. Primers and probes were chosen based on the consensus sequences of gag and pol clones representative of EV1 genetic variants. Both PCRs had a detection limit of 3 copies of target gene, with a linearity over 6 orders of magnitude. The performances of the two PCRs in vivo were evaluated and compared on a panel of DNAs extracted from blood of sheep infected experimentally with EV1. The pol assay detected in most cases lower numbers of viral molecules than gag assay, yielding some false negative results. The gag real-time RT PCR had a detection limit of 100 RNA molecules with a linearity over 5 orders of magnitude. This did not result in a lower performance of the RT PCR compared to the PCR in cells permissive for virus replication, which contain higher numbers of viral transcripts than proviral genomes. The real-time assays developed in this study, particularly the gag assay, provide a sensitive tool which can be used to quantify the viral load in experimental infections. Copyright 2010 Elsevier B.V. All rights reserved.Entities:
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Year: 2010 PMID: 20116400 DOI: 10.1016/j.jviromet.2010.01.013
Source DB: PubMed Journal: J Virol Methods ISSN: 0166-0934 Impact factor: 2.014