Prospective Multicenter Clinical Evaluation of AMPLICOR and COBAS AMPLICOR Hepatitis C Virus Tests

Author:

Nolte Frederick S.1,Fried Michael W.2,Shiffman Mitchell L.3,Ferreira-Gonzalez Andrea4,Garrett Carlton T.4,Schiff Eugene R.5,Polyak Stephen J.6,Gretch David R.6

Affiliation:

1. Department of Pathology and Laboratory Medicine, Emory University School of Medicine, Atlanta, Georgia1;

2. Division of Hepatology, University of North Carolina School of Medicine, Chapel Hill, North Carolina2;

3. Hepatology Section3 and

4. Department of Pathology,4 Medical College of Virginia Commonwealth University, Richmond, Virginia;

5. Division of Hepatology, University of Miami School of Medicine, Miami, Florida5; and

6. Department of Laboratory Medicine, University of Washington School of Medicine, Seattle, Washington6

Abstract

ABSTRACT We conducted a multicenter clinical evaluation of the second versions of the manual AMPLICOR and the semiautomated COBAS AMPLICOR tests for hepatitis C virus (HCV) RNA (Roche Molecular Systems, Inc., Pleasanton, Calif.). The performance characteristics of these HCV RNA tests for diagnosis of active viral infection were determined by comparison to anti-HCV serological test results, alanine aminotransferase levels, and liver biopsy histology results. A total of 878 patients with clinical or biochemical evidence of liver disease were enrolled at four hepatology clinics. A total of 1,089 specimens (901 serum and 188 plasma) were tested with the AMPLICOR test. Sensitivity compared to serology was 93.1% for serum and 90.6% for plasma. The specificity was 97% for serum and 93.1% for plasma. A total of 1,084 specimens (896 serum and 188 plasma) were tested with the COBAS test. Sensitivities for serum and plasma were the same as with the AMPLICOR test. The specificity was 97.8% for serum and 96.6% for plasma. Of the 69 specimens with false-positive and false-negative AMPLICOR test results relative to those of serology, alternative primer set (APS) reverse transcription (RT)-PCR analysis showed that the AMPLICOR test provided the correct result relative to the specimens containing HCV RNA in 64 (92.7%) specimens. Similarly, 66 of 67 (98.5%) false-positive and false-negative COBAS test results were determined to be correct by APS RT-PCR analysis. There were no substantive differences in clinical performances between study sites, patient groups, specimen types, storage conditions (−20 to −80°C versus 2 to 8°C), or anticoagulants (EDTA versus acid citrate dextrose) for either test. Both tests showed >99% reproducibility within runs, within sites, and overall. We conclude that these tests can reliably detect the presence of HCV RNA, as evidence of active infection, in patients with clinical or biochemical evidence of liver disease.

Publisher

American Society for Microbiology

Subject

Microbiology (medical)

Reference20 articles.

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2. Sequence analysis of the core gene of 14 hepatitis C virus genotypes;Bukh J.;Proc. Natl. Acad. Sci. USA,1994

3. Recommendations for prevention and control of hepatitis C virus (HCV) infection and HCV-related chronic disease;Centers for Disease Control and Prevention;Morb. Mortal. Wkly. Rep.,1998

4. International collaborative study on the second EUROHEP HCV-RNA reference panel;Damen M.;J. Virol. Methods,1996

5. Second Generation of the Automated Cobas Amplicor HCV Assay Improves Sensitivity of Hepatitis C Virus RNA Detection and Yields Results That Are More Clinically Relevant

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