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通过多重Luminex检测法同时定量检测人乳头瘤病毒6型、11型、16型和18型病毒样颗粒上中和表位的抗体。

Simultaneous quantitation of antibodies to neutralizing epitopes on virus-like particles for human papillomavirus types 6, 11, 16, and 18 by a multiplexed luminex assay.

作者信息

Opalka David, Lachman Charles E, MacMullen Stefani A, Jansen Kathrin U, Smith Judith F, Chirmule Narendra, Esser Mark T

机构信息

Virus and Cell Biology, Merck Research Laboratories, Wayne, Pennsylvania 19087-8630, USA.

出版信息

Clin Diagn Lab Immunol. 2003 Jan;10(1):108-15. doi: 10.1128/cdli.10.1.108-115.2003.

DOI:10.1128/cdli.10.1.108-115.2003
PMID:12522048
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC145272/
Abstract

Several different methods have been developed to quantitate neutralizing antibody responses to human papillomaviruses (HPVs), including in vivo neutralization assays, in vitro pseudoneutralization assays, competitive radioimmunoassays (cRIAs), and enzyme-linked immunosorbent assays. However, each of these techniques possesses one or more limitations that preclude testing large numbers of patient sera for use in natural history studies and large vaccine clinical trials. We describe here a new multiplexed assay, by using the Luminex Laboratory MultiAnalyte Profiling (LabMAP3) assay system, that can simultaneously quantitate neutralizing antibodies to human papillomavirus types 6, 11, 16, and 18 in 50 micro l of serum. The HPV-Luminex competitive immunoassay measures titers of polyclonal antibodies in serum capable of displacing phycoerythrin-labeled detection monoclonal antibodies binding to conformationally sensitive, neutralizing epitopes on the respective virus-like particles. This competitive Luminex immunoassay was found to be as sensitive, accurate, and precise as the currently used cRIAs. An effective HPV vaccine will most likely require several distinct genotypes to protect against multiple cancer causing papillomaviruses. The HPV-Luminex immunoassay should prove to be a useful tool in simultaneously quantitating antibody immune responses to multiple HPV genotypes for natural history infection studies and for monitoring the efficacy of prospective vaccines.

摘要

已经开发出几种不同的方法来定量针对人乳头瘤病毒(HPV)的中和抗体反应,包括体内中和试验、体外假中和试验、竞争性放射免疫测定(cRIA)和酶联免疫吸附测定。然而,这些技术中的每一种都有一个或多个局限性,这使得无法对大量患者血清进行检测以用于自然史研究和大型疫苗临床试验。我们在此描述一种新的多重检测方法,通过使用Luminex实验室多分析物分析(LabMAP3)检测系统,该系统可以在50微升血清中同时定量针对人乳头瘤病毒6型、11型、16型和18型的中和抗体。HPV-Luminex竞争性免疫测定法可测量血清中多克隆抗体的滴度,这些抗体能够取代与各自病毒样颗粒上构象敏感的中和表位结合的藻红蛋白标记的检测单克隆抗体。发现这种竞争性Luminex免疫测定法与目前使用的cRIA一样灵敏、准确和精确。一种有效的HPV疫苗很可能需要几种不同的基因型来预防多种致癌乳头瘤病毒。HPV-Luminex免疫测定法应该会被证明是一种有用的工具,可同时定量针对多种HPV基因型的抗体免疫反应,用于自然史感染研究和监测前瞻性疫苗的疗效。

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