| Literature DB >> 21871496 |
Carlos Santos1, Alexanda Reis, Cintia Vilhena Dos Santos, Cristine Damas, Mariliza Henrique Silva, Mônica Valverde Viana, Maria Lucia Ferraz, Dimas Carnauba, Fabiane El-Far, Fernando Serra, Ricardo Sobhie Diaz.
Abstract
Collecting and transporting samples for RNA analysis can be challenging, especially in situations where financial resources are limited. In this study, a quantitative real-time PCR (qPCR) for the analysis of HCV RNA was developed and adapted for use with dried blood spot (DBS) samples. A qPCR for HCV 5'NCR, an internal control and a calibration curve were developed, and the sensitivity, specificity and dynamic range of amplification were evaluated using a panel of viruses. Plasma and DBS samples from 100 patients who had completed four weeks of Peginterferon alfa-2b+Ribavirin treatment were collected (DBS on SS903 collection cards and transported at room temperature). After 24 weeks of treatment, samples were collected from 68 of these patients. Of the 168 samples, 2 yielded false-negative results, and 4 yielded false-positive results (sensitivity was 98%, specificity was 94.3%, positive predictive value was 96.1%, and negative predictive value was 96.9%). Additionally, 2039 DBS samples from 1114 patients currently undergoing treatment for a chronic HCV infection in a clinical trial were tested. Only 10 samples out of the 2039 yielded invalid results warranting re-collection of DBS. The detection of HCV RNA in DBS can be a cost-effective strategy for HCV treatment monitoring, especially in settings where resources are limited.Entities:
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Year: 2011 PMID: 21871496 DOI: 10.1016/j.jviromet.2011.06.012
Source DB: PubMed Journal: J Virol Methods ISSN: 0166-0934 Impact factor: 2.014