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慢病毒整合酶功能性四聚体化的结构基础

Structural basis for functional tetramerization of lentiviral integrase.

作者信息

Hare Stephen, Di Nunzio Francesca, Labeja Alfred, Wang Jimin, Engelman Alan, Cherepanov Peter

机构信息

Division of Medicine, St. Mary's Campus, Imperial College London, London, United Kingdom.

出版信息

PLoS Pathog. 2009 Jul;5(7):e1000515. doi: 10.1371/journal.ppat.1000515. Epub 2009 Jul 17.

Abstract

Experimental evidence suggests that a tetramer of integrase (IN) is the protagonist of the concerted strand transfer reaction, whereby both ends of retroviral DNA are inserted into a host cell chromosome. Herein we present two crystal structures containing the N-terminal and the catalytic core domains of maedi-visna virus IN in complex with the IN binding domain of the common lentiviral integration co-factor LEDGF. The structures reveal that the dimer-of-dimers architecture of the IN tetramer is stabilized by swapping N-terminal domains between the inner pair of monomers poised to execute catalytic function. Comparison of four independent IN tetramers in our crystal structures elucidate the basis for the closure of the highly flexible dimer-dimer interface, allowing us to model how a pair of active sites become situated for concerted integration. Using a range of complementary approaches, we demonstrate that the dimer-dimer interface is essential for HIV-1 IN tetramerization, concerted integration in vitro, and virus infectivity. Our structures moreover highlight adaptable changes at the interfaces of individual IN dimers that allow divergent lentiviruses to utilize a highly-conserved, common integration co-factor.

摘要

实验证据表明,整合酶(IN)四聚体是协同链转移反应的主角,通过该反应逆转录病毒DNA的两端被插入宿主细胞染色体中。在此,我们展示了两个晶体结构,其中包含梅迪-维斯纳病毒IN的N端和催化核心结构域,并与常见慢病毒整合辅助因子LEDGF的IN结合结构域形成复合物。这些结构表明,IN四聚体的二聚体-二聚体结构通过在准备执行催化功能的内部单体对之间交换N端结构域而得以稳定。我们晶体结构中四个独立的IN四聚体的比较阐明了高度灵活的二聚体-二聚体界面闭合的基础,使我们能够模拟一对活性位点如何定位以进行协同整合。使用一系列互补方法,我们证明二聚体-二聚体界面对于HIV-1 IN四聚化、体外协同整合和病毒感染性至关重要。此外,我们的结构突出了各个IN二聚体界面处的适应性变化,这些变化使不同的慢病毒能够利用高度保守的共同整合辅助因子。

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