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开发并评估一种简单有效的 RT-qPCR 抑制分析方法,用于检测化合物对 HIV 逆转录酶的抑制效果。

Development and evaluation of a simple and effective RT-qPCR inhibitory assay for detection of the efficacy of compounds towards HIV reverse transcriptase.

机构信息

IRCCS Centro Neurolesi "Bonino-Pulejo", Messina, Italy.

Department of Chemical, Biological, Pharmaceutical, and Environmental Sciences, University of Messina, Via F. Stagno d'Alcontres 31, 98166, Messina, Italy.

出版信息

Appl Microbiol Biotechnol. 2017 Nov;101(22):8249-8258. doi: 10.1007/s00253-017-8544-6. Epub 2017 Sep 30.

DOI:10.1007/s00253-017-8544-6
PMID:28963576
Abstract

Assessing the actual efficacy of compounds to directly inhibit HIV reverse transcriptase (RT) activity is a main goal in preclinical antiretroviral studies. Our previous studies demonstrated that the effects of inhibitor compounds towards HIV-RT could be efficiently assessed through a simple cell-free assay based on conventional reverse transcription PCR. In the present study, we describe a modified variant of our assay, termed RT real-time quantitative PCR inhibitory assay (RT-qPCR-IA), in which the ability of compounds to restrict the complementary DNA (cDNA) generation by HIV-RT using a specific RNA template is performed by the real-time technique, in order to improve both accuracy and sensitivity of the method. As specific RNA template, RNA extracted from stable transfectants ectopically expressing the herpes simplex virus 1 glycoprotein D gene was utilized. HIV-RT, of both commercial or house-made viral lysate origin, was employed for the assay. To assess the reliability of RT-qPCR-IA, we performed a comparative, quantitative analysis of the dose-dependent effect exerted by known nucleotide and non-nucleotide reverse-transcriptase inhibitors, using the SYBR Green dye chemistry as detection system. The results obtained with RT-qPCR-IA were compared to that obtained using a one-step PicoGreen technology-based commercial kit. The outcome of our study indicates that the development of the novel RT-qPCR-IA will provide rapid and accurate evaluation of the inhibitory efficacy of compounds towards HIV-RT activity. This evaluation could be very useful for large-scale screening of potential new anti-HIV drugs.

摘要

评估化合物直接抑制 HIV 逆转录酶 (RT) 活性的实际疗效是临床前抗逆转录病毒研究的主要目标。我们之前的研究表明,通过基于常规逆转录 PCR 的简单无细胞测定,可以有效地评估抑制剂化合物对 HIV-RT 的作用。在本研究中,我们描述了我们的测定法的一种改良变体,称为 RT 实时定量 PCR 抑制测定法 (RT-qPCR-IA),其中化合物通过实时技术限制 HIV-RT 利用特定 RNA 模板生成互补 DNA(cDNA)的能力,以提高方法的准确性和灵敏度。作为特定的 RNA 模板,使用从稳定转染的外源性表达单纯疱疹病毒 1 糖蛋白 D 基因的细胞中提取的 RNA。使用商业或自制病毒裂解物来源的 HIV-RT 进行测定。为了评估 RT-qPCR-IA 的可靠性,我们使用 SYBR Green 染料化学作为检测系统,对已知核苷酸和非核苷酸逆转录酶抑制剂的剂量依赖性作用进行了定量分析。使用基于一步 PicoGreen 技术的商业试剂盒获得的结果与 RT-qPCR-IA 获得的结果进行了比较。我们的研究结果表明,新型 RT-qPCR-IA 的开发将为化合物对 HIV-RT 活性的抑制效果提供快速、准确的评估。这种评估对于大规模筛选潜在的新型抗 HIV 药物非常有用。

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