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质粒RSF1010六聚体复制解旋酶RepA的晶体结构。

Crystal structure of the hexameric replicative helicase RepA of plasmid RSF1010.

作者信息

Niedenzu T, Röleke D, Bains G, Scherzinger E, Saenger W

机构信息

Institut für Kristallographie, Freie Universität Berlin, Takustr. 6, Berlin, D-14195, Germany.

出版信息

J Mol Biol. 2001 Feb 23;306(3):479-87. doi: 10.1006/jmbi.2000.4398.

DOI:10.1006/jmbi.2000.4398
PMID:11178907
Abstract

Unwinding of double-stranded DNA into single-stranded intermediates required for various fundamental life processes is catalyzed by helicases, a family of mono-, di- or hexameric motor proteins fueled by nucleoside triphosphate hydrolysis. The three-dimensional crystal structure of the hexameric helicase RepA encoded by plasmid RSF1010 has been determined by X-ray diffraction at 2.4 A resolution. The hexamer shows an annular structure with 6-fold rotational symmetry and a approximately 17 A wide central hole, suggesting that single-stranded DNA may be threaded during unwinding. Homologs of all five conserved sequence motifs of the DnaB-like helicase family are found in RepA, and the topography of the monomer resembles RecA and the helicase domain of the bacteriophage T7 gp4 protein. In a modeled complex, ATP molecules are located at the subunit interfaces and clearly define adenine-binding and ATPase catalytic sites formed by amino acid residues located on adjacent monomers; most remarkable is the "arginine finger" Arg207 contributing to the active site in the adjacent monomer. This arrangement of active-site residues suggests cooperativity between monomers in ATP hydrolysis and helicase activity of RepA. The mechanism of DNA unwinding remains elusive, as RepA is 6-fold symmetric, contrasting the recently published asymmetric structure of the bacteriophage T7 gp4 helicase domain.

摘要

解旋酶催化双链DNA解旋成各种基本生命过程所需的单链中间体,解旋酶是一类由核苷三磷酸水解提供能量的单体、二聚体或六聚体驱动蛋白家族。通过X射线衍射在2.4埃分辨率下确定了质粒RSF1010编码的六聚体解旋酶RepA的三维晶体结构。该六聚体呈现出具有6倍旋转对称性的环状结构和一个宽约17埃的中心孔,这表明单链DNA在解旋过程中可能会穿过该孔。在RepA中发现了DnaB样解旋酶家族所有五个保守序列基序的同源物,其单体的拓扑结构类似于RecA和噬菌体T7 gp4蛋白的解旋酶结构域。在一个模拟复合物中,ATP分子位于亚基界面处,并清晰地界定了由相邻单体上的氨基酸残基形成的腺嘌呤结合位点和ATP酶催化位点;最引人注目的是“精氨酸指”Arg207对相邻单体中的活性位点有贡献。活性位点残基的这种排列表明RepA在ATP水解和解旋酶活性方面单体之间存在协同作用。由于RepA是六倍对称的,这与最近发表的噬菌体T7 gp4解旋酶结构域的不对称结构形成对比,DNA解旋的机制仍然难以捉摸。

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