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开发和评估一种经济实惠的实时定性检测方法,用于确定血浆和干血斑中 HIV-1 病毒学失败。

Development and evaluation of an affordable real-time qualitative assay for determining HIV-1 virological failure in plasma and dried blood spots.

机构信息

University Medical Centre Utrecht, Utrecht, the Netherlands.

出版信息

J Clin Microbiol. 2013 Jun;51(6):1899-905. doi: 10.1128/JCM.03305-12. Epub 2013 Apr 17.

DOI:10.1128/JCM.03305-12
PMID:23596235
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3716048/
Abstract

Virological failure (VF) has been identified as the earliest, most predictive determinant of HIV-1 antiretroviral treatment (ART) failure. Due to the high cost and complexity of virological monitoring, VF assays are rarely performed in resource-limited settings (RLS). Rather, ART failure is determined by clinical monitoring and to a large extent immunological monitoring. This paper describes the development and evaluation of a low-cost, dried blood spot (DBS)-compatible qualitative assay to determine VF, in accordance with current WHO guideline recommendations for therapy switching in RLS. The assay described here is an internally controlled qualitative real-time PCR targeting the conserved long terminal repeat domain of HIV-1. This assay was applied to HIV-1 subtypes A to H and further evaluated on HIV-1 clinical plasma samples from South Africa (n = 191) and Tanzania (n = 42). Field evaluation was performed in Uganda using local clinical plasma samples (n = 176). Furthermore, assay performance was evaluated for DBS. This assay is able to identify VF for all major HIV-1 group M subtypes with equal specificity and has a lower detection limit of 1.00E+03 copies/ml for plasma samples and 5.00E+03 copies/ml for DBS. Comparative testing yielded accurate VF determination for therapy switching in 89% to 96% of samples compared to gold standards. The assay is robust and flexible, allowing for "open platform" applications and producing results comparable to those of commercial assays. Assay design enables application in laboratories that can accommodate real-time PCR equipment, allowing decentralization of testing to some extent. Compatibility with DBS extends access of sampling and thus access to this test to remote settings.

摘要

病毒学失败(VF)已被确定为 HIV-1 抗逆转录病毒治疗(ART)失败的最早和最具预测性的决定因素。由于病毒学监测的成本高且复杂,资源有限环境(RLS)很少进行 VF 检测。相反,ART 失败是通过临床监测和在很大程度上免疫监测来确定的。本文描述了一种低成本、干血斑(DBS)兼容的定性检测方法的开发和评估,该方法符合当前 RLS 中治疗转换的世卫组织指南建议,用于确定 VF。本文描述的检测方法是针对 HIV-1 的保守长末端重复区域的内部对照定性实时 PCR。该检测方法适用于 HIV-1 亚型 A 至 H,并进一步在南非(n = 191)和坦桑尼亚(n = 42)的 HIV-1 临床血浆样本中进行评估。在乌干达使用当地临床血浆样本(n = 176)进行了现场评估。此外,还评估了 DBS 对检测的影响。该检测方法能够识别所有主要 HIV-1 组 M 亚型的 VF,具有相同的特异性,其对血浆样本的检测下限为 1.00E+03 拷贝/ml,对 DBS 的检测下限为 5.00E+03 拷贝/ml。与金标准相比,比较测试在 89%至 96%的样本中能够准确确定 VF,从而进行治疗转换。该检测方法具有稳健性和灵活性,允许“开放式平台”应用,并产生与商业检测方法相当的结果。该检测方法的设计允许在可以容纳实时 PCR 设备的实验室中应用,在一定程度上实现了检测的分散化。与 DBS 的兼容性扩展了采样的机会,从而使偏远地区也能获得该检测。

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