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HIV-1 RT 引物-模板复合物的 MD 模拟:修饰核苷和反义 PNA 寡聚物的影响。

MD simulations of HIV-1 RT primer-template complex: effect of modified nucleosides and antisense PNA oligomer.

机构信息

Centre for Development of Advanced Computing, Pune University Campus, Pune, 411007, India.

出版信息

J Biomol Struct Dyn. 2013;31(6):539-60. doi: 10.1080/07391102.2012.706076. Epub 2012 Aug 13.

DOI:10.1080/07391102.2012.706076
PMID:22888964
Abstract

Human immunodeficiency virus type 1 (HIV-1) requires the human tRNA(3)(Lys) as a reverse transcriptase (RT) primer. The annealing of 3' terminal 18 nucleotides of tRNA(3)(Lys) with the primer binding site (PBS) of viral RNA (vRNA) is crucial for reverse transcription. Additional contacts between the A rich (A-loop) region of vRNA and the anticodon domain of tRNA(3)(Lys) are necessary, which show the specific requirement of tRNA(3)(Lys). The importance of modified nucleosides, present in tRNA(3)(Lys), in giving stability to the primer-template complex has been determined in earlier experiments. It has been observed that the PNA oligomer targeted to PBS of vRNA destabilized the crucial interactions between primer and template due to which the reverse transcription is inhibited. Molecular dynamics simulations have been carried out to study the effect of modified nucleosides on the vRNA-tRNA(3)(Lys) complex stability and the destabilization effect of PNA oligomer on the vRNA-tRNA(3)(Lys)-PNA complex. The root-mean-square deviation, hydrogen bonding, tertiary interactions, and free energy calculations of the simulation data support the experimental results. The analyses have revealed the structural changes in PBS region of vRNA which might be another strong reason for the inability of RT binding to 7F helix for its normal functioning of reverse transcription.

摘要

人类免疫缺陷病毒 1 型 (HIV-1) 需要人 tRNA(3)(Lys) 作为逆转录酶 (RT) 的引物。tRNA(3)(Lys)的 3'末端 18 个核苷酸与病毒 RNA (vRNA)的引物结合位点 (PBS) 的退火对于逆转录至关重要。vRNA 的 A 丰富 (A-环) 区域与 tRNA(3)(Lys)的反密码子结构域之间的额外接触是必要的,这表明 tRNA(3)(Lys)的特异性要求。在早期实验中已经确定了存在于 tRNA(3)(Lys)中的修饰核苷对引物-模板复合物稳定性的重要性。已经观察到针对 vRNA PBS 的 PNA 寡聚体由于破坏了引物和模板之间的关键相互作用,从而抑制了逆转录。已经进行了分子动力学模拟,以研究修饰核苷对 vRNA-tRNA(3)(Lys)复合物稳定性的影响,以及 PNA 寡聚体对 vRNA-tRNA(3)(Lys)-PNA 复合物的去稳定化作用。模拟数据的均方根偏差、氢键、三级相互作用和自由能计算支持实验结果。分析揭示了 vRNA 的 PBS 区域的结构变化,这可能是 RT 无法结合 7F 螺旋以正常进行逆转录的另一个重要原因。

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