Three commercially available 3rd-generation anti-HCV ELISAs (Abbott, Murex and Ortho) were evaluated in various serum panels: (A) blood donor samples (n = 403) with 1st- or 2nd-generation anti-HCV ELISA (various manufacturers) positive test results; (B) non-A, non-B hepatitis patients (n = 212); (C) multi- transfused patients (n = 253); (D) serial dilutions of HCV confirmed (RIBA and PCR) positive blood donors (n = 24), and (E) first-time blood donors (n = 1,055). All samples of panels A, B and C were tested in PCR and RIBA-2. In panels A, B and C, 398 samples were HCV PCR positive: all were detected by Abbott and Ortho, and 397 (99.7%) by Murex. The sample missed by the Murex ELISA showed an isolated anti-C33c reactivity in RIBA-2. In panels A-C, 442 samples were RIBA-2 positive and all were detected by the 3 tests. With Probit analysis on results of panel D, no significant difference in sensitivity was observed between the 3 evaluated ELISAs. Specificities of Abbott, Murex and Ortho in 1,055 blood donors were 99.7, 99.3 and 99.9%, respectively (NS, χ2). We conclude that the sensitivity and specificity of the 3 ELISAs are comparable although the C33c antigen in the Murex VK47 test should be improved.
Aim: Evaluation of a qualitative HTLV-I/Il DNA polymerase chain reaction
(PCR) test for the detection of HTLV-I/II DNA (Roche Diagnostic Systems,
Branchburg, N.J., USA) in various panels. Methods: The panels consisted of
fresh EDTA blood samples from blood donors who were anti-HTLV-I/II ELISA
repeatably reactive: 53 were Western blot (WB) positive, 228 were WB indeterminate
and 15 were WB negative. Elevent ELISA-negative blood donors were
used as negative controls. Furthermore, specimens from 1 HTLV-II-infected intravenous
drug user and from 1 HTLV-II-infected blood donor were included in
the panel. Peripheral blood lymphocytes were prepared by red blood cell lysis
with the Roche washing solution and stored at <-23 °C until processing. Amplification
products were analyzed with the HTLV-I/II detection kit. Results: All
53 anti-HTLV-I/II ELISA- and WB-positive samples and both HTLV-II-positive
samples tested positively by PCR. All 228 anti-HTLV-I/II ELISA-positive and
WB-indeterminate, all 15 ELISA-positive and WB-negative and all 11 ELISAnegative
control samples tested negative by PCR. Conclusion: The Roche Amplicor
HTLV-I/II test is a simple test, suitable for the confirmation of HTLV-I and
-II infection in individuals with indeterminate or positive WB patterns.
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