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A novel, cell-free PCR-based assay for evaluating the inhibitory activity of antiretroviral compounds against HIV reverse transcriptase

机译:一种新颖的,无细胞的基于PCR的测定方法,用于评估抗逆转录病毒化合物对HIV逆转录酶的抑制活性

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摘要

This study describes a novel, PCR-based assay that evaluates the ability of compounds to inhibit cDNA generation by HIV reverse transcriptase (RT), of both commercial and viral lysate origin, from a known RNA template. The template consisted of RNA from stable transfectants ectopically expressing the US6 gene of herpes simplex virus-1, coding for glycoprotein D. Controls were carried out to demonstrate that no residual DNA polymerase activity or DNA contamination was responsible for the amplified DNA in the tested, control samples. In this assay, 0.1μM nevirapine totally inhibited the RT activity of 0.5U commercial HIV RT, while 10nM inhibited it by only 10%. Conversely, 10pM efavirenz completely inhibited 0.5U HIV RT. Similar results were obtained when a self-prepared viral lysate was used as a source of HIV RT. A reference commercial kit directly measuring HIV RT activity, without amplification, was less sensitive than the new assay. As a consequence, the HIV RT 50% inhibitory concentration of nevirapine and efavirenz in the newly described assay was 8 and 5×103 times lower, respectively, than in the commercial assay. In conclusion, this novel method was sensitive, reproducible, and sufficiently rapid for screening in vitro the functional activity of known or potential antiretroviral compounds against HIV RT.
机译:这项研究描述了一种新颖的基于PCR的检测方法,该方法可从已知的RNA模板评估化合物抑制商业和病毒裂解物来源的HIV逆转录酶(RT)产生cDNA的能力。模板由来自稳定转染子的RNA组成,该转染子从异位表达单纯疱疹病毒1的US6基因,编码糖蛋白D。进行了对照实验,证明在测试的扩增DNA中没有残留的DNA聚合酶活性或DNA污染,对照样品。在该分析中,0.1μM奈韦拉平完全抑制了0.5U商业HIV RT的RT活性,而10nM仅抑制了10%。相反,10pM依非韦伦可完全抑制0.5U HIV RT。当使用自行制备的病毒裂解液作为HIV RT来源时,可获得相似的结果。直接测量HIV RT活性而不进行扩增的参考商业试剂盒比新检测方法灵敏。结果,在新描述的测定中,奈韦拉平和依非韦伦的HIV RT 50%抑制浓度分别比市售测定低8和5×103倍。总之,该新方法灵敏,可重现,并且足够快,可以在体外筛选已知或潜在的抗逆转录病毒化合物针对HIV RT的功能活性。

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