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位点特异性重组酶结构与功能的准等价性:与三向Lox DNA接头结合的三聚体Cre重组酶的晶体结构及活性

Quasi-equivalence in site-specific recombinase structure and function: crystal structure and activity of trimeric Cre recombinase bound to a three-way Lox DNA junction.

作者信息

Woods K C, Martin S S, Chu V C, Baldwin E P

机构信息

Section of Molecular and Cellular Biology, University of California, Davis, 1 Shields Ave, Davis, CA 95616, USA.

出版信息

J Mol Biol. 2001 Oct 12;313(1):49-69. doi: 10.1006/jmbi.2001.5012.

DOI:10.1006/jmbi.2001.5012
PMID:11601846
Abstract

The crystal structure of a novel Cre-Lox synapse was solved using phases from multiple isomorphous replacement and anomalous scattering, and refined to 2.05 A resolution. In this complex, a symmetric protein trimer is bound to a Y-shaped three-way DNA junction, a marked departure from the pseudo-4-fold symmetrical tetramer associated with Cre-mediated LoxP recombination. The three-way DNA junction was accommodated by a simple kink without significant distortion of the adjoining DNA duplexes. Although the mean angle between DNA arms in the Y and X structures was similar, adjacent Cre trimer subunits rotated 29 degrees relative to those in the tetramers. This rotation was accommodated at the protein-protein and DNA-DNA interfaces by interactions that are "quasi-equivalent" to those in the tetramer, analogous to packing differences of chemically identical viral subunits at non-equivalent positions in icosahedral capsids. This structural quasi-equivalence extends to function as Cre can bind to, cleave and perform strand transfer with a three-way Lox substrate. The structure explains the dual recognition of three and four-way junctions by site-specific recombinases as being due to shared structural features between the differently branched substrates and plasticity of the protein-protein interfaces. To our knowledge, this is the first direct demonstration of quasi-equivalence in both the assembly and function of an oligomeric enzyme.

摘要

利用多重同晶置换和反常散射得到的相位信息,解析了一种新型Cre-Lox突触的晶体结构,并将其精修至2.05埃分辨率。在这个复合物中,一个对称的蛋白质三聚体与一个Y形三链DNA连接点结合,这与Cre介导的LoxP重组相关的假四倍对称四聚体有显著不同。三链DNA连接点通过一个简单的扭结得以容纳,相邻的DNA双链没有明显扭曲。虽然Y形和X形结构中DNA臂之间的平均角度相似,但相邻的Cre三聚体亚基相对于四聚体中的亚基旋转了29度。这种旋转通过与四聚体中“准等效”的相互作用在蛋白质-蛋白质和DNA-DNA界面得以实现,类似于二十面体衣壳中化学相同的病毒亚基在非等效位置的堆积差异。这种结构上的准等效性延伸到功能上,因为Cre可以与三链Lox底物结合、切割并进行链转移。该结构解释了位点特异性重组酶对三链和四链连接点的双重识别,这是由于不同分支底物之间共享的结构特征以及蛋白质-蛋白质界面的可塑性所致。据我们所知,这是寡聚酶组装和功能中准等效性的首次直接证明。

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Quasi-equivalence in site-specific recombinase structure and function: crystal structure and activity of trimeric Cre recombinase bound to a three-way Lox DNA junction.位点特异性重组酶结构与功能的准等价性:与三向Lox DNA接头结合的三聚体Cre重组酶的晶体结构及活性
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