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基于血清标本混合检测的人类免疫缺陷病毒感染血清流行病学调查准确且具有成本效益吗?

Are seroepidemiological surveys for human immunodeficiency virus infection based on tests on pools of serum specimens accurate and cost-effective?

作者信息

Parry J V, Mahoney A, Mortimer P P

机构信息

Hepatitis and Retrovirus Laboratory, PHLS Virus Reference Division, Central Public Health Laboratory, London, UK.

出版信息

Clin Diagn Virol. 1993 Aug;1(3):167-78. doi: 10.1016/0928-0197(93)90011-s.

Abstract

Serum specimens (n = 17668) from UK antenatal patients in the Thames Regions were tested by Wellcozyme HIV 1/2 EIA singly and in pools of 6, 12 and 24: 35 (0.2%, 1 in 505) were confirmed as anti-HIV positive. The pools of 12 were also tested for anti-HIV 1/2 by IAF Biochem, Behring and Diagnostics Pasteur EIAs. All 35 positive specimens were easily detectable after pooling in groups of 12. The false positive rate for Wellcozyme was nearly halved compared with individual testing (1 in 309 false positive compared with 1 in 174). For the other assays false positive rates on pools of 12 were: IAF Biochem 1 in 193, Behring 1 in 140, Diagnostics Pasteur 1 in 1547. Twenty-two known anti-HIV 2-positive sera were detected by all four EIAs when diluted as in pools of 6 and 12, but by only three EIAs in pools of 24 and 48. Pooling in groups of 6 did not seem to delay detection of HIV 1 seroconversion, but pooling in groups of 12, 24 and 48 might delay it by 1, 2 and 3 weeks respectively. For this study the effect of pooling in groups of 12 would have been a reagent saving of 87-91% and a labour saving of about 50%. Because of the low HIV incidence and rarity of specimens collected around seroconversion in UK, little, if any, loss of sensitivity would result from it. Pooling in groups of 12 has therefore been chosen for the screening of anonymous antenatal specimens in the UK.

摘要

对泰晤士地区英国产前患者的血清样本(n = 17668)进行了检测,先用Wellcozyme HIV 1/2酶免疫分析单独检测,然后再以6份、12份和24份样本为一组进行混合检测:35份(0.2%,即1/505)被确认为抗HIV阳性。12份样本一组的混合样本还用IAF Biochem、贝林和巴斯德诊断公司的酶免疫分析检测了抗HIV 1/2。所有35份阳性样本在12份一组混合后都很容易检测出来。与单独检测相比,Wellcozyme的假阳性率几乎减半(单独检测时为1/174出现假阳性,混合检测时为1/309出现假阳性)。对于其他检测方法,12份样本一组混合检测时的假阳性率分别为:IAF Biochem为1/193,贝林为1/140,巴斯德诊断公司为1/1547。22份已知抗HIV 2阳性血清在按6份和12份样本一组稀释时,四种酶免疫分析均能检测到,但在按24份和48份样本一组稀释时,只有三种酶免疫分析能检测到。6份样本一组混合检测似乎不会延迟HIV 1血清转化的检测,但12份、24份和48份样本一组混合检测可能分别会延迟1周、2周和3周。在本研究中,12份样本一组混合检测可节省87 - 91%的试剂和约50%的人力。由于英国HIV发病率较低且血清转化前后采集的样本很少见,因此这样做几乎不会导致敏感性损失。因此,英国已选择12份样本一组混合检测来筛查匿名产前样本。

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