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在使用特定抗逆转录病毒化合物治疗期间对1型人类免疫缺陷病毒活性进行定量分子监测。

Quantitative molecular monitoring of human immunodeficiency virus type 1 activity during therapy with specific antiretroviral compounds.

作者信息

Bagnarelli P, Menzo S, Valenza A, Paolucci S, Petroni S, Scalise G, Sampaolesi R, Manzin A, Varaldo P E, Clementi M

机构信息

Institute of Microbiology, University of Ancona, Italy.

出版信息

J Clin Microbiol. 1995 Jan;33(1):16-23. doi: 10.1128/jcm.33.1.16-23.1995.

Abstract

Methods for the absolute quantitation of nucleic acids present in small amounts in biological samples (competitive PCR and competitive reverse transcription PCR) were applied to the direct monitoring of specific anti-human immunodeficiency virus type 1 (HIV-1) therapy. With these techniques, different parameters of HIV-1 activity (including genomic RNA copy numbers in plasma, proviral and late transcript copy numbers in peripheral blood lymphocytes, and mean transcriptional activity per each HIV-1 provirus) were monitored during therapy with azidothymidine or ddI. In most of these treated patients, a direct response to the antiretroviral compounds employed was detected during the first few weeks of treatment, as documented by a fast decrease of all molecular indexes of HIV-1 activity. However, residual viral replication (albeit at minimal levels) was documented during therapy in all subjects monitored in this study. In a minority of the patients under study (3 of 12), the drug-dependent viral inhibition was maintained throughout the observation time (213 to 791 days), but in 9 patients a rebound in viremia level was detected during therapy with competitive reverse transcription PCR. Sequencing analysis of a portion of the HIV-1 gene pol from cell-free virions showed that circulating viral variants bearing at least two mutations compatible with azidothymidine or ddI resistance were detectable in the patients who exhibited a rebound in cell-free HIV-1 genomic RNA copy numbers in plasma but not in one patient who maintained (for 455 days) lowered levels of viral load during ddI treatment.

摘要

将用于对生物样品中少量存在的核酸进行绝对定量的方法(竞争性PCR和竞争性逆转录PCR)应用于直接监测特异性抗人免疫缺陷病毒1型(HIV-1)治疗。利用这些技术,在使用叠氮胸苷或双脱氧肌苷治疗期间,监测HIV-1活性的不同参数(包括血浆中的基因组RNA拷贝数、外周血淋巴细胞中的前病毒和晚期转录本拷贝数,以及每个HIV-1前病毒的平均转录活性)。在这些接受治疗的大多数患者中,在治疗的最初几周内就检测到了对所用抗逆转录病毒化合物的直接反应,这通过HIV-1活性的所有分子指标快速下降得以证明。然而,在本研究监测的所有受试者的治疗期间,都记录到了残余的病毒复制(尽管水平极低)。在所研究的少数患者(12例中的3例)中,药物依赖性病毒抑制在整个观察期(213至791天)内持续存在,但在9例患者中,在竞争性逆转录PCR治疗期间检测到病毒血症水平反弹。对来自无细胞病毒颗粒的HIV-1基因pol的一部分进行测序分析表明,在血浆中无细胞HIV-1基因组RNA拷贝数出现反弹的患者中可检测到携带至少两个与叠氮胸苷或双脱氧肌苷抗性相容的突变的循环病毒变体,但在一名在双脱氧肌苷治疗期间(455天)维持低病毒载量水平的患者中未检测到。

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