Germer J J, Rys P N, Thorvilson J N, Persing D H
Division of Experimental Pathology, Mayo Clinic, Rochester, Minnesota 55905, USA.
J Clin Microbiol. 1999 Aug;37(8):2625-30. doi: 10.1128/JCM.37.8.2625-2630.1999.
Consistent with other members of the family Flaviviridae, hepatitis C virus (HCV) demonstrates a high degree of sequence variation throughout the coding regions of its genome. However, there is a high degree of sequence conservation found within the 5' untranslated region (UTR) of the genome, making this region a target of choice for most nucleic acid amplification-based detection assays. In this study, the Amplicor HCV test, a commercially available assay which detects the 5'UTR, was used for the detection of HCV RNA in 669 serum samples obtained from a cohort of liver transplantation patients. Amplification products obtained from the HCV-positive cases were subjected to direct sequencing and genotyping based upon seven phylogenetically informative regions within the 5'UTR. Of the 669 specimens, 416 (62.2%) tested positive for the presence of HCV RNA. Of these, 372 (89.4%) specimens were successfully classified into 11 HCV genotypes and subtypes after computer-assisted analysis of the sequence data. Forty-four (10.6%) of the HCV RNA-positive specimens were not classifiable, the majority corresponding to low-titer specimens as determined by the Chiron Quantiplex HCV RNA 2. 0 assay. Additional comparative studies targeting the NS-5 region of the viral genome generally confirmed the accuracy and sensitivity of the 5'UTR-based classifications, with the exception of the misclassification of a small number of type 1a cases as type 1b. We conclude that although the high sequence conservation within the 5'UTR results in the misclassification of a small number of HCV subtypes, the overall gains of efficiency, the shorter turnaround time, the inclusion of contamination control measures, and the low rate of test failure compared to that of methods based on the NS-5 gene together constitute significant advantages over other techniques.
与黄病毒科的其他成员一致,丙型肝炎病毒(HCV)在其基因组的编码区域表现出高度的序列变异。然而,在基因组的5'非翻译区(UTR)发现了高度的序列保守性,使得该区域成为大多数基于核酸扩增的检测方法的首选目标。在本研究中,使用一种市售的检测5'UTR的Amplicor HCV检测法,对从一组肝移植患者获得的669份血清样本中的HCV RNA进行检测。从HCV阳性病例获得的扩增产物基于5'UTR内的七个系统发育信息区域进行直接测序和基因分型。在669个标本中,416个(62.2%)检测出HCV RNA阳性。其中,372个(89.4%)标本在对序列数据进行计算机辅助分析后成功分类为11种HCV基因型和亚型。44个(10.6%)HCV RNA阳性标本无法分类,大多数对应于Chiron Quantiplex HCV RNA 2.0检测法确定的低滴度标本。针对病毒基因组NS-5区域的其他比较研究总体上证实了基于5'UTR分类的准确性和敏感性,但有少数1a型病例被误分类为1b型。我们得出结论,尽管5'UTR内的高度序列保守性导致少数HCV亚型被误分类,但与基于NS-5基因的方法相比,效率的整体提高、周转时间的缩短、污染控制措施的纳入以及低检测失败率共同构成了相对于其他技术的显著优势。