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HIV-1核衣壳在核酸底物上捕获逆转录酶。

HIV-1 nucleocapsid traps reverse transcriptase on nucleic acid substrates.

作者信息

Grohmann Dina, Godet Julien, Mély Yves, Darlix Jean-Luc, Restle Tobias

机构信息

Institut Gilbert Laustriat, Photophysique des interactions moleculaires, UMR 7175 CNRS, Faculte de Pharmacie, Universite Louis Pasteur, Strasbourg 1, 74, Route du Rhin, 67401 Illkirch, France.

出版信息

Biochemistry. 2008 Nov 18;47(46):12230-40. doi: 10.1021/bi801386r. Epub 2008 Oct 24.

DOI:10.1021/bi801386r
PMID:18947237
Abstract

Conversion of the genomic RNA of human immunodeficiency virus (HIV) into full-length viral DNA is a complex multistep reaction catalyzed by the reverse transcriptase (RT). Numerous studies have shown that the viral nucleocapsid (NC) protein has a vital impact on various steps during reverse transcription, which is crucial for virus infection. However, the exact molecular details are poorly defined. Here, we analyzed the effect of NC on RT-catalyzed single-turnover, single-nucleotide incorporation using different nucleic acid substrates. In the presence of NC, we observed an increase in the amplitude of primer extension of up to 3-fold, whereas the transient rate of nucleotide incorporation ( k pol) dropped by up to 50-fold. To unravel the underlying molecular mechanism, we carefully analyzed the effect of NC on RT-nucleic acid substrate dissociation. The studies revealed that NC considerably enhances the stability of RT-substrate complexes by reducing the observed dissociation rate constants, which more than compensates for the observed drop in k pol. In conclusion, our data strongly support the concept that NC not only indirectly assists the reverse transcription process by its nucleic acid chaperoning activity but also positively affects the RT-catalyzed nucleotide incorporation reaction by increasing polymerase processivity presumably via a physical interaction of the two viral proteins.

摘要

人类免疫缺陷病毒(HIV)的基因组RNA转化为全长病毒DNA是一个由逆转录酶(RT)催化的复杂多步反应。大量研究表明,病毒核衣壳(NC)蛋白在逆转录过程的各个步骤中都具有至关重要的影响,这对病毒感染至关重要。然而,确切的分子细节仍不清楚。在这里,我们使用不同的核酸底物分析了NC对RT催化的单轮单核苷酸掺入的影响。在存在NC的情况下,我们观察到引物延伸幅度增加了高达3倍,而核苷酸掺入的瞬时速率(k pol)下降了高达50倍。为了揭示潜在的分子机制,我们仔细分析了NC对RT-核酸底物解离的影响。研究表明,NC通过降低观察到的解离速率常数,大大提高了RT-底物复合物的稳定性,这足以弥补观察到的k pol下降。总之,我们的数据有力地支持了这样一个概念,即NC不仅通过其核酸伴侣活性间接协助逆转录过程,而且可能通过两种病毒蛋白的物理相互作用增加聚合酶的持续合成能力,从而对RT催化的核苷酸掺入反应产生积极影响。

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