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用于检测丙型肝炎病毒抗体的第二代和第三代酶免疫测定法的比较

Comparison of second- and third-generation enzyme immunoassays for detecting antibodies to hepatitis C virus.

作者信息

Abdel-Hamid Mohamed, El-Daly Mai, El-Kafrawy Sherif, Mikhail Nabiel, Strickland G Thomas, Fix Alan D

机构信息

Hepatitis C Project, Egypt, International Health Division, University of Maryland School of Medicine, 660 West Redwood Street, Baltimore, MD 21201, USA.

出版信息

J Clin Microbiol. 2002 May;40(5):1656-9. doi: 10.1128/JCM.40.5.1656-1659.2002.

Abstract

Supplemental assays, such as recombinant immunoblot assays (RIBA), are used to confirm detection of antibodies to hepatitis C virus (HCV). However, due to their expense, they are not widely used in developing countries. The purpose of our study was to compare the results of second- and third-generation (G2 and G3, respectively) enzyme immunoassays (EIAs) and to resolve discordant results by using a supplemental assay to assess the reliability of G2 and G3 EIAs to confirm anti-HCV antibody-positive results. We performed both G2 and G3 EIAs for anti-HCV antibodies on 1,134 serum samples collected during the 2nd year of a longitudinal community-based study in Egypt; 35 samples with discordant results were tested by Abbott Laboratories Micro-Particle Immunoassay (M-EIA) and RIBA. Viremia was determined with an in-house nested reverse transcriptase PCR (RT-PCR) to detect HCV RNA. Concordance between the two assays (G2/G3) was 96.9%; 87 (7.7%) samples were positive and 1,012 (89.2%) were negative by both assays. For 17 samples, the discordant results were G2 assay negative and G3 assay positive, and for 18 samples, the discordant results were G2 assay positive and G3 assay negative. Among the 17 G2 assay-negative and G3 assay-positive samples, 15 were M-EIA positive and 7 were PCR positive. Among the 18 G2 assay-positive and G3 assay-negative samples, 2 were M-EIA positive and none were PCR positive. RIBA results from 24 discordant samples showed 87.5% agreement with the G3 EIA, 12.5% agreement with the G2 EIA, and 95.8% agreement with M-EIA. Eleven samples were indeterminate by RIBA and excluded from this analysis. Based on RIBA results, the sensitivity of the G3 EIA was 99%, compared to 89.8% for the G2 EIA, while the specificity of the G3 EIA was 99.8%, compared to 98.9% for the G2 EIA. These results show that the reliability of the G3 EIA in screening these sera is excellent, and the G3 assay can be used in the absence of supplemental tests where resources are limited. RIBA appears not to have advantages over the less expensive M-EIA screening assay. The main disadvantage of RIBA is the occurrence of indeterminate results, especially among problematic samples. Samples giving discordant results in multiple assays are often indeterminate with the RIBA.

摘要

补充检测,如重组免疫印迹检测(RIBA),用于确认丙型肝炎病毒(HCV)抗体的检测。然而,由于其成本较高,在发展中国家并未广泛使用。我们研究的目的是比较第二代和第三代(分别为G2和G3)酶免疫测定(EIA)的结果,并通过使用补充检测来解决不一致的结果,以评估G2和G3 EIA确认抗HCV抗体阳性结果的可靠性。我们对在埃及一项基于社区的纵向研究的第二年收集的1134份血清样本进行了G2和G3抗HCV抗体EIA检测;35份结果不一致的样本通过雅培实验室微粒子免疫测定(M-EIA)和RIBA进行检测。采用内部巢式逆转录聚合酶链反应(RT-PCR)测定病毒血症以检测HCV RNA。两种检测方法(G2/G3)之间的一致性为96.9%;两种检测方法均显示87份(7.7%)样本为阳性,1012份(89.2%)样本为阴性。对于17份样本,不一致的结果是G2检测为阴性而G3检测为阳性,对于18份样本,不一致的结果是G2检测为阳性而G3检测为阴性。在17份G2检测阴性且G3检测阳性的样本中,15份M-EIA检测为阳性,7份PCR检测为阳性。在18份G2检测阳性且G3检测阴性的样本中,2份M-EIA检测为阳性,无PCR检测为阳性。24份结果不一致样本的RIBA结果显示,与G3 EIA的一致性为87.5%,与G2 EIA的一致性为12.5%,与M-EIA的一致性为95.8%。11份样本RIBA结果不确定,被排除在该分析之外。基于RIBA结果,G3 EIA的敏感性为99%,而G2 EIA为89.8%,同时G3 EIA的特异性为99.8%,而G2 EIA为98.9%。这些结果表明,G3 EIA在筛查这些血清方面的可靠性极佳,并且在资源有限且没有补充检测的情况下,G3检测可被使用。RIBA似乎并不比成本较低的M-EIA筛查检测具有优势。RIBA的主要缺点是出现不确定结果,尤其是在有问题的样本中。在多种检测中结果不一致的样本,RIBA检测结果往往不确定。

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