Literature DB >> 8386692

Quantitation of hepatitis C virus RNA in serum of asymptomatic blood donors and patients with type C chronic liver disease.

H Hagiwara1, N Hayashi, E Mita, M Naito, A Kasahara, H Fusamoto, T Kamada.   

Abstract

We describe a method for quantifying hepatitis C virus RNA in serum. This competitive assay combines reverse transcription and polymerase chain reaction and is based on coamplification of the target RNA with known amounts of synthetic mutated RNA. We tested serum samples from 104 hepatitis C virus carriers (9 asymptomatic blood donors and 95 patients with type C chronic liver disease) to determine the relationship between the replicative level of hepatitis C virus and various stages of the carrier states. The amount of circulating hepatitis C virus RNA ranged from 10(4) to 10(9.5) genomes/ml serum. The titer of hepatitis C virus RNA (logarithmic transformed copy numbers of RNA per milliliter of serum) was lower in asymptomatic blood donors (5.4 +/- 2.0) and in patients with chronic persistent hepatitis (7.3 +/- 1.1) than in patients with chronic active hepatitis (7.9 +/- 0.8), cirrhosis (7.8 +/- 0.7) or hepatocellular carcinoma (7.9 +/- 0.7). The titer of hepatitis C virus RNA was significantly lower in carriers younger than 40 yr old and correlated positively with the logarithmic transformed serum ALT level. Logistic regression showed that age and titer of hepatitis C virus RNA correlated independently with the stages of liver disease. These results showed that the replicative level of hepatitis C virus is higher in advanced liver disease and that elevation of viral replication may play an important role in liver injury and progression of liver disease. This competitive assay is useful in evaluating the state of viral replication in hepatitis C virus infection.

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Year:  1993        PMID: 8386692     DOI: 10.1002/hep.1840170404

Source DB:  PubMed          Journal:  Hepatology        ISSN: 0270-9139            Impact factor:   17.425


  32 in total

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3.  Influence of human immunodeficiency virus type 1 infection on the natural course of chronic parenterally acquired hepatitis C.

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Journal:  Eur J Clin Microbiol Infect Dis       Date:  1995-11       Impact factor: 3.267

4.  Comparison of two quantitative hepatitis C virus reverse transcriptase PCR assays.

Authors:  W K Roth; J H Lee; B Rüster; S Zeuzem
Journal:  J Clin Microbiol       Date:  1996-02       Impact factor: 5.948

5.  Prospective multicenter clinical evaluation of AMPLICOR and COBAS AMPLICOR hepatitis C virus tests.

Authors:  F S Nolte; M W Fried; M L Shiffman; A Ferreira-Gonzalez; C T Garrett; E R Schiff; S J Polyak; D R Gretch
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6.  Long-term biochemical and virological response to natural interferon-alpha in patients with chronic hepatitis C.

Authors:  H Hagiwara; N Hayashi; A Kasahara; M Oshita; K Katayama; M Naito; M Masuzawa; H Yoshihara; Y Shimizu; H Fusamoto; T Kamada
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7.  Immunological evaluation in oral lichen planus with chronic hepatitis C.

Authors:  Y Nagao; M Sata; K Abe; K Tanikawa; T Kameyama
Journal:  J Gastroenterol       Date:  1997-06       Impact factor: 7.527

8.  Comparative evaluation of the total hepatitis C virus core antigen, branched-DNA, and amplicor monitor assays in determining viremia for patients with chronic hepatitis C during interferon plus ribavirin combination therapy.

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9.  Chronic hepatitis C virus infections: predictive value of genotype and level of viraemia on disease progression and response to interferon alpha.

Authors:  J C Booth; G R Foster; U Kumar; R Galassini; R D Goldin; J L Brown; H C Thomas
Journal:  Gut       Date:  1995-03       Impact factor: 23.059

10.  Quantification of hepatitis C virus RNA by competitive amplification of RNA from denatured serum and hybridization on microtiter plates.

Authors:  A Ravaggi; A Zonaro; C Mazza; A Albertini; E Cariani
Journal:  J Clin Microbiol       Date:  1995-02       Impact factor: 5.948

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