COMPARISON OF QUANTITATIVE CDNA-PCR WITH THE BRANCHED DNA HYBRIDIZATION ASSAY FOR MONITORING PLASMA HEPATITIS-C VIRUS-RNA LEVELS IN HEMOPHILIA PATIENTS PARTICIPATING IN A CONTROLLED INTERFERON TRIAL

被引:39
作者
BRESTERS, D
CUYPERS, HTM
REESINK, HW
MAUSERBUNSCHOTEN, EP
VANDENBERG, HM
SCHAASBERG, WP
WILBER, JC
URDEA, MS
NEUWALD, P
LELIE, PN
机构
[1] NETHERLANDS RED CROSS,BLOOD BANK,AMSTERDAM,NETHERLANDS
[2] UNIV UTRECHT HOSP,VAN CREVELD CLIN,UTRECHT,NETHERLANDS
[3] CHIRON CORP,EMERYVILLE,CA
关键词
HCV; IFN; QUANTITATION;
D O I
10.1002/jmv.1890430313
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
The branched DNA (bDNA) assay was compared with a semi-quantitative cDNA-polymerase chain reaction (cDNA-PCR) assay for monitoring HCV RNA levels in plasma in 17 haemophilia patients participating in a controlled cr-interferon trial. Good correlation between the HCV RNA levels as detected by the two assays was observed, with a correlation co-efficient of 0.83 (P < 0.0001) and 0.90 (P < 0.0001) at week 0 and 24, respectively. Hepatitis C virus RNA (HCV RNA) levels could be assessed with the bDNA assay in 14/17 (82 percent) HCV cDNA-PCR positive pretreatment samples. The bDNA assay apparently failed to detect low viral titres. Interferon treated patients (n = 11) showed either a complete response, being a large reduction in HCV RNA level to below the detection limit of the HCV cDNA-PCR assay (6/11) or no significant reduction in HCV RNA level (5/11). A ''partial'' virological response was not observed. The changes in HCV RNA plasma levels in non-responders during interferon (IFN) treatment were similar to the (small) natural fluctuations in viral load observed in controls (untreated patients). Although the bDNA assay was not as sensitive as cDNA-PCR, given its user friendliness and quantitative results, it is concluded that it is a useful test for monitoring HCV RNA levels in patients treated with interferon. However, patients who are nonreactive in the bDNA assay have to be retested by cDNA-PCR because low viral titres are not detected by the bDNA assay. (C) 1994 Wiley-Liss, Inc.
引用
收藏
页码:262 / 268
页数:7
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