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人类免疫缺陷病毒1型核衣壳蛋白p7与模型RNA的结合特性:功能结构决定因素的阐明

Binding properties of the human immunodeficiency virus type 1 nucleocapsid protein p7 to a model RNA: elucidation of the structural determinants for function.

作者信息

Urbaneja M A, Kane B P, Johnson D G, Gorelick R J, Henderson L E, Casas-Finet J R

机构信息

AIDS Vaccine Program, SAIC Frederick, National Cancer Institute-Frederick Cancer Research and Development Center, Frederick, MD, 21702-1201, USA.

出版信息

J Mol Biol. 1999 Mar 19;287(1):59-75. doi: 10.1006/jmbi.1998.2521.

DOI:10.1006/jmbi.1998.2521
PMID:10074407
Abstract

HIV-1 nucleocapsid protein (NCp7) is a double zinc-fingered protein that has been traditionally implicated in viral RNA recognition and packaging, in addition to its tight association with genomic RNA and tRNA primer within the virion nucleocapsid. The availability of large quantities of viral or recombinant wild-type NCp7 and mutant p7 has made possible the assignment of the different roles that structural motifs within the protein play during RNA binding. At low ionic strength binding to the homopolymeric fluorescent RNA, poly(epsilonA), is electrostatically driven and four sodium ions are displaced. Arg7 in the flanking N-terminal region, Lys20 and Lys26 in the first zinc finger and one positively charged residue (attributed to Lys41) in the second zinc finger are involved in electrostatic contacts with RNA. The p7 zinc fingers do not function independently but concomitantly. The first zinc finger (both isolated or in the context of the full-length protein) has a more prominent electrostatic interaction than the second one. The second zinc finger dominates the non-electrostatic stabilization of the binding to RNA due to stacking of its Trp residue with nucleic acid bases. Mutations in the highly conserved retroviral Zn-coordinating residues (CCHC) to steroid hormone receptor (CCCC) or transcription factor (CCHH) metal cluster types do not affect RNA binding. In spite of the limited impact in RNA binding affinity in vitro or RNA packaging in vivo that such mutations or structural alterations impart, they impair or abolish virus infectivity. It is likely that such an effect stems from the involvement of NCp7 in crucial steps of the virus life cycle other than RNA binding.

摘要

HIV-1核衣壳蛋白(NCp7)是一种双锌指蛋白,除了在病毒粒子核衣壳内与基因组RNA和tRNA引物紧密结合外,传统上还参与病毒RNA的识别和包装。大量病毒或重组野生型NCp7及突变体p7的可得性,使得确定该蛋白内结构基序在RNA结合过程中所起的不同作用成为可能。在低离子强度下,与同聚荧光RNA聚(εA)的结合是由静电驱动的,并且有四个钠离子被置换。侧翼N端区域的Arg7、第一个锌指中的Lys20和Lys26以及第二个锌指中的一个带正电荷残基(归因于Lys41)参与与RNA的静电接触。p7锌指并非独立发挥作用,而是协同作用。第一个锌指(无论是分离的还是全长蛋白中的)比第二个锌指具有更显著的静电相互作用。第二个锌指由于其色氨酸残基与核酸碱基的堆积,在与RNA结合的非静电稳定中起主导作用。将高度保守的逆转录病毒锌配位残基(CCHC)突变为类固醇激素受体(CCCC)或转录因子(CCHH)金属簇类型,并不影响RNA结合。尽管此类突变或结构改变在体外对RNA结合亲和力或体内对RNA包装的影响有限,但它们会损害或消除病毒感染性。这种效应很可能源于NCp7参与了病毒生命周期中除RNA结合之外的关键步骤。

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