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在携带不同地理来源毒株的患者中评估的HIV-1诊断性PCR引物标准化及算法。比利时艾滋病参考实验室。

Standardisation of primers and an algorithm for HIV-1 diagnostic PCR evaluated in patients harbouring strains of diverse geographical origin. The Belgian AIDS Reference Laboratories.

作者信息

Vandamme A M, Fransen K, Debaisieux L, Marissens D, Sprecher S, Vaira D, Vandenbroucke A T, Verhofstede C

机构信息

Katholieke Universiteit Leuven, Rega Instituut, Belgium.

出版信息

J Virol Methods. 1995 Feb;51(2-3):305-16. doi: 10.1016/0166-0934(94)00126-2.

DOI:10.1016/0166-0934(94)00126-2
PMID:7738151
Abstract

Eight Belgian AIDS Reference Laboratories established a multicentre quality control to evaluate the performance of their diagnostic human immunodeficiency virus type 1 (HIV-1) DNA polymerase chain reaction (PCR). A set of Belgian and African HIV-1 seropositive and seronegative patient samples, collected in Belgium, and the British Medical Research Council (MRC) HIV-1 PCR reference reagent kit, containing plasmid HIV-1 DNA at several dilutions in human carrier DNA with appropriate negative controls, were tested by the laboratories. No false positive results were reported. All laboratories were able to detect one to two copies of HIV-1 DNA. Among the 17 Belgian and African HIV-1 seropositives, some laboratories reported up to four indeterminate results, mainly due to failure of the SK38-39, SK68-69 (Ou et al. (1988) Science 239, 295-297) and/or gag881-882 (Simmonds et al. (1990) J. Virol. 64, 864-872) primers and a poorly performing algorithm. Only the H1POL4235-4538 nested pol primer set, developed by one of the laboratories, correctly identified all the tested HIV-1 positive and negative samples. Consequently, the laboratories decided to evaluate these pol primers as a reference primer set and to standardise the testing algorithm. All laboratories achieved a sensitivity and specificity of 100% on testing 10 additional Belgian and African patient samples, when adapting a standardised algorithm based on three HIV-1 primer sets, one of which is the H1POL4235-4538 primer set.

摘要

比利时的八家艾滋病参考实验室建立了一项多中心质量控制措施,以评估其诊断人类免疫缺陷病毒1型(HIV-1)DNA聚合酶链反应(PCR)的性能。这些实验室对一组在比利时采集的比利时和非洲HIV-1血清阳性和血清阴性患者样本,以及英国医学研究理事会(MRC)的HIV-1 PCR参考试剂试剂盒进行了检测。该试剂盒包含在人类载体DNA中几种稀释度的质粒HIV-1 DNA以及适当的阴性对照。未报告有假阳性结果。所有实验室都能够检测到一到两个HIV-1 DNA拷贝。在17份比利时和非洲HIV-1血清阳性样本中,一些实验室报告了多达四个不确定结果,主要是由于SK38-39、SK68-69(Ou等人,(1988年)《科学》239卷,295 - 297页)和/或gag881-882(Simmonds等人,(1990年)《病毒学杂志》64卷,864 - 872页)引物失败以及算法性能不佳。只有其中一个实验室开发的H1POL4235-4538巢式pol引物组正确鉴定了所有检测的HIV-1阳性和阴性样本。因此,这些实验室决定将这些pol引物评估为参考引物组并标准化检测算法。当采用基于三种HIV-1引物组(其中之一是H1POL4235-4538引物组)的标准化算法时,所有实验室在检测另外10份比利时和非洲患者样本时均达到了100%的灵敏度和特异性。

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