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为马拉维卡龙加麻风病疫苗试验开展艾滋病毒血清学检测。

Setting up HIV serology for the Karonga leprosy vaccine trial in Malaŵi.

作者信息

Shaw M A, Turner A C, Blackwell J M, Fine P E, Ponnighaus J M

机构信息

London School of Hygiene and Tropical Medicine.

出版信息

Lepr Rev. 1991 Mar;62(1):87-104. doi: 10.5935/0305-7518.19910012.

Abstract

As part of the leprosy vaccine trial taking place in Karonga District, Northern Malaŵi, it is essential to establish whether the presence of HIV infection in the population is affecting the incidence rate or clinical presentation of leprosy or the effectiveness of the trial vaccines. To obtain the appropriate information, a rapid and economical HIV testing protocol, which could be performed in a rural laboratory and would be robust under variable environmental conditions, had to be developed. This paper reports on the development/evaluation phase of a multitest protocol based on commercially available particle agglutination and ELISA anti-HIV antibody detection kits. The protocol was devised by first evaluating a range of kits in London using a battery of African and non-African sera and then field testing 1455 sera in Malaŵi, which included 184 sera from leprosy patients and 60 sera from syphilis patients to check for cross-reactivity. According to the protocol developed, all sera are screened initially both by indirect ELISA (Organon) and using a rapid and economical modification of the Serodia particle agglutination test. Positives are retested using both a competitive ELISA (Wellcome or Behring) and the standard Serodia particle agglutination test. The validity of this multitest protocol was confirmed by Western blotting a large sample of the positive and negative Malaŵian sera in London. Factors affecting kit selection, and problems associated with individual kits, are discussed. While the specific multitest protocol developed for Malaŵi might not be suitable for every project, the principle of developing economical alternatives to Western blotting is an important consideration for any field investigation of HIV.

摘要

作为在马拉维北部卡龙加区开展的麻风疫苗试验的一部分,确定该人群中艾滋病毒感染的存在是否正在影响麻风的发病率、临床表现或试验疫苗的有效性至关重要。为了获取适当的信息,必须制定一种快速且经济的艾滋病毒检测方案,该方案可在农村实验室进行,并且在各种环境条件下都能稳定运行。本文报告了一种基于市售颗粒凝集和ELISA抗艾滋病毒抗体检测试剂盒的多重检测方案的开发/评估阶段。该方案的设计过程是,首先在伦敦使用一系列非洲和非非洲血清对一系列试剂盒进行评估,然后在马拉维对1455份血清进行现场检测,其中包括184份麻风患者血清和60份梅毒患者血清,以检查交叉反应性。根据制定的方案,所有血清首先通过间接ELISA(欧加农公司产品)以及对血清学颗粒凝集试验进行快速且经济的改良方法进行筛查。阳性样本使用竞争ELISA(威康或贝林公司产品)和标准血清学颗粒凝集试验进行重新检测。通过在伦敦对大量马拉维阳性和阴性血清样本进行蛋白质印迹法,证实了该多重检测方案的有效性。文中讨论了影响试剂盒选择的因素以及与各个试剂盒相关的问题。虽然为马拉维制定的特定多重检测方案可能并不适用于每个项目,但开发蛋白质印迹法经济替代方法的原则对于任何艾滋病毒现场调查都是一个重要的考虑因素。

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