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Single-molecule studies on the role of HIV-1 nucleocapsid protein/nucleic acid interaction in the viral replication cycle.

机译:HIV-1核衣壳蛋白/核酸相互作用在病毒复制周期中作用的单分子研究。

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摘要

The discovery of the crucial intermediates and pathway in the process of the reverse transcription was reported using single-molecule spectroscopy and related techniques including single-molecule fluorescence resonance energy transfer, fluorescence correlation spectroscopy and confocal imaging. Reverse transcription of the HIV-1 RNA genome involves several complex nucleic acid rearrangement steps that are catalyzed by the HIV-1 nucleocapsid protein (NC), including for example, the annealing of the transactivation response (TAR) region of the viral RNA to the complementary region (TAR DNA) in minus-strand strong-stop DNA. In this dissertation, the research focused on elucidating the mechanism of NC-facilitated TAR DNA/RNA annealing. The single molecule spectroscopic measurements reported that the crucial intermediates as well as the mechanistic insight into the annealing of TAR RNA with TAR DNA mediated by viral NC proteins. The data reveal that NC partially melted the secondary structure of TAR DNA (termed the "YTAR") as well as TAR RNA. In the subsequent studies, various short DNA oligonucleotdies were applied to anneal with the TAR to mimic the initial annealing steps. The data support that the YTAR serves as a nucleation center for the annealing to occur through the multiple sites along the TAR structure. Two major nucleation pathways were observed, which are the annealing through the 3'/5' termini, namely "zipper" pathway and the annealing through the hairpin loop region, namely "kissing" pathway. The annealing mechanism was further explored by performing the annealing of wild-type TAR DNA with wild-type TAR RNA in the presence of NC in vitro. The annealing kinetic data suggest that the nucleation of TAR DNA/RNA annealing occurs in an encounter complex form in which one or two DNA/RNA strands in the "Y" form associated with multiple NC molecules. This encounter complex leads to the multiple nucleation complexes, i.e. zipper or kissing intermediates. The data further indicate that although the two complementary strands nucleate at multiple sites, i.e. any single-strand region of TAR, the annealing of two TAR complements occurs through a common mechanism.
机译:使用单分子光谱法和相关技术(包括单分子荧光共振能量转移,荧光相关光谱法和共聚焦成像)报道了逆转录过程中关键中间体和途径的发现。 HIV-1 RNA基因组的逆转录涉及被HIV-1核衣壳蛋白(NC)催化的几个复杂的核酸重排步骤,包括例如病毒RNA的反式激活反应(TAR)区的退火。负链强终止DNA中的互补区(TAR DNA)。本文的研究重点是阐明数控促进TAR DNA / RNA退火的机制。单分子光谱测量法报道了关键中间体以及由病毒NC蛋白介导的TAR DNA与TAR DNA退火的机理研究。数据表明,NC部分融化了TAR DNA(称为“ YTAR”)和TAR RNA的二级结构。在随后的研究中,将各种短DNA寡核苷酸应用于TAR退火,以模拟初始退火步骤。数据支持将YTA​​R用作成核中心,使退火沿着TAR结构的多个位置发生。观察到两个主要成核途径,即通过3'/ 5'末端的退火,即“拉链”途径和通过发夹环区域的退火,即“亲吻”途径。通过在NC存在下对野生型TAR DNA和野生型TAR RNA进行退火来进一步探索退火机制。退火动力学数据表明,TAR DNA / RNA退火的成核以相遇复杂形式发生,其中“ Y”形的一或两条DNA / RNA链与多个NC分子相关。这种相遇复合物导致多个成核复合物,即拉链或接吻中间体。数据进一步表明,尽管两条互补链在多个位点(即TAR的任何单链区域)成核,但是两个TAR互补序列的退火通过共同机制发生。

著录项

  • 作者

    Liu, Hsiao-Wei.;

  • 作者单位

    The University of Texas at Austin.$bChemistry.;

  • 授予单位 The University of Texas at Austin.$bChemistry.;
  • 学科 Chemistry Biochemistry.; Chemistry Physical.; Biology Virology.
  • 学位 Ph.D.
  • 年度 2007
  • 页码 132 p.
  • 总页数 132
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 生物化学;物理化学(理论化学)、化学物理学;
  • 关键词

  • 入库时间 2022-08-17 11:40:29

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