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一种检测具有转录活性的1型人类免疫缺陷病毒颗粒的检测方法的开发。

Development of an assay that detects transcriptionally competent human immunodeficiency virus type one particles.

作者信息

Busso M, Resnick L

机构信息

Retrovirology Research Department, Mount Sinai Medical Center, Miami Beach, FL 33140.

出版信息

J Virol Methods. 1994 Apr;47(1-2):129-39. doi: 10.1016/0166-0934(94)90072-8.

Abstract

To study the functional properties of HIV-1 reverse transcriptase (RT) from intact viral particles without the requirement for tissue culture expansion, a method that couples HIV-1 reverse transcription utilizing its endogenous RT (ERT) with polymerase chain reaction amplification (PCR) was developed. Detection of endogenous reverse transcripts from HIV particles by ERT-PCR was compared to HIV RNA PCR detection using avian myeloblastosis virus (AMV) RT from plasma samples from 45 HIV-1 infected patients. The HIV ERT-PCR method was capable of detecting plasma viremia with the same efficiency (29/29 patients) as the AMV RT HIV RNA PCR in patients with CD4 cell counts of less than 500/mm3. The determination of HIV-RT drug sensitivities using four well-characterized HIV-1 lab strains was assessed. The ERT-PCR method detected reduced sensitivity to TIBO R82150 (10 microM) in a TIBO resistant strain but not in the TIBO sensitive HTLV-IIIB viral mixture or an HTLV-IIIB clone. In summary, the HIV ERT-PCR method provides a useful approach for the detection of HIV and the characterization of RT sensitivities among HIV-1 strains.

摘要

为了研究完整病毒颗粒中HIV-1逆转录酶(RT)的功能特性,且无需进行组织培养扩增,开发了一种将利用其内源RT(ERT)的HIV-1逆转录与聚合酶链反应扩增(PCR)相结合的方法。通过ERT-PCR检测HIV颗粒中的内源逆转录产物,并与使用来自45例HIV-1感染患者血浆样本中的禽成髓细胞瘤病毒(AMV)RT进行的HIV RNA PCR检测进行比较。在CD4细胞计数低于500/mm3的患者中,HIV ERT-PCR方法检测血浆病毒血症的效率与AMV RT HIV RNA PCR相同(29/29例患者)。评估了使用四种特征明确的HIV-1实验室菌株测定HIV-RT药物敏感性的情况。ERT-PCR方法在一株对TIBO耐药的菌株中检测到对TIBO R82150(10 microM)的敏感性降低,但在对TIBO敏感的HTLV-IIIB病毒混合物或HTLV-IIIB克隆中未检测到。总之,HIV ERT-PCR方法为检测HIV以及表征HIV-1菌株之间RT敏感性提供了一种有用的方法。

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