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Journal of Clinical Microbiology, Oct 1996, 2552-2558, Vol 34, No. 10
F Umlauft, DT Wong, PJ Oefner, PA Underhill, RC Cheung, TL Wright, AA Kolykhalov, K Gruenewald and HB Greenberg
A single-round PCR method with primers specific for the 3' noncoding region
(NCR) of hepatitis C virus (HCV) has been developed. Using a double
RNAzol-B extraction, a high-temperature reverse-transcription step with
SuperScript II reverse transcriptase, and a 40-cycle two- temperature PCR
with a TaqStart antibody hot-start procedure, we were able to detect a
92-nucleotide fragment of the recently discovered 98- nucleotide highly
conserved sequence at the 3' terminus of the HCV genome. Direct sequencing
of the PCR products confirmed the specificity of the PCR and demonstrated
conservation in this region. Only one nucleotide change in 14 specimens was
found. End point dilution titration of sera with known viral RNA titers
showed the sensitivity of the single-round 3' NCR PCR to be comparable to
those of the established nested 5' NCR assays (fewer than 25 HCV genome
equivalents). To evaluate specificity and sensitivity, a panel of 116 serum
samples characterized by nested 5'-end PCR, genotyping, and quantitative
assays was tested. A high degree of concordance (96%) between the 3' NCR
and 5' NCR PCR results was found. The sequence conservation at the 3' end
of the HCV genome among common genotypes and the savings in time, labor,
and reagents from a single-round PCR make this assay a useful addition to
the detection systems available to identify and monitor HCV infection.
Copyright © 1996 by the American Society for Microbiology. All rights reserved.
Hepatitis C virus detection by single-round PCR specific for the terminal 3' noncoding region
Division of Gastroenterology, Stanford University, California 94305, USA.
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