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Absolute quantitation of viremia in human immunodeficiency virus infection by competitive reverse transcription and polymerase chain reaction.

机译:通过竞争性逆转录和聚合酶链反应对人类免疫缺陷病毒感染中的病毒血症进行绝对定量。

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摘要

A competitive polymerase chain reaction (PCR)-based assay for the quantitative detection of human immunodeficiency virus type 1 (HIV-1) viremia was developed and optimized. This method consists of the reverse transcription and subsequent amplification in the same tube of two similar RNA templates, the wild-type template to be quantified and a known amount of the internally deleted synthetic template, both with identical primer recognition sites. The same strategy also proved to be useful in the quantitative assay of HIV-1-specific cellular transcripts and proviral DNA sequences from peripheral blood mononuclear cells by using competitor DNA. The method might be of interest in the study of the precise level of HIV-1 activity during the different clinical phases of the infection and in the simple, fast, and methodologically correct molecular investigation of patients treated with specific antiviral compounds.
机译:开发并优化了一种基于竞争性聚合酶链反应(PCR)的定量检测人类免疫缺陷病毒1型(HIV-1)病毒血症的检测方法。该方法由两个相似的RNA模板(待定量的野生型模板)和已知量的内部缺失的合成模板(均具有相同的引物识别位点)在同一试管中进行逆转录和随后的扩增组成。通过使用竞争者DNA,同样的策略也被证明可用于HIV-1特异性细胞转录物和外周血单核细胞的原病毒DNA序列的定量分析。该方法可能对研究感染的不同临床阶段中HIV-1活性的精确水平以及对用特定抗病毒化合物治疗的患者进行的简单,快速和方法正确的分子研究感兴趣。

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