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与34碱基对切割位点复合的位点特异性重组酶γδ解离酶的晶体结构。

Crystal structure of the site-specific recombinase gamma delta resolvase complexed with a 34 bp cleavage site.

作者信息

Yang W, Steitz T A

机构信息

Department of Molecular Biophysics and Biochemistry, Yale University, New Haven, Connecticut 06520, USA.

出版信息

Cell. 1995 Jul 28;82(2):193-207. doi: 10.1016/0092-8674(95)90307-0.

Abstract

The structure of gamma delta resolvase complexed with a 34 bp substrate DNA has been determined at 3.0 A resolution. The DNA is sharply bent by 60 degrees toward the major groove and away from the resolvase catalytic domains at the recombination crossover point. The C-terminal one third of resolvase, which was disordered in the absence of DNA, forms an arm and a 3-helix DNA-binding domain on the opposite side of the DNA from the N-terminal domain. The arms wrap around the minor groove of the central 16 bp, and the DNA-binding domains interact with the major grooves near the outer boundaries of the binding site. The resolvase dimer is asymmetric, particularly in the arm region, implying a conformational adaptability that may be important for resolvase binding to different DNA sites in the synaptosome. It also raises the possibility of a sequential single-strand cleavage mechanism.

摘要

已在3.0埃分辨率下确定了与34碱基对底物DNA复合的γδ解离酶的结构。在重组交叉点处,DNA向大沟急剧弯曲60度,并远离解离酶催化结构域。解离酶的C端三分之一在没有DNA时是无序的,在DNA与N端结构域相对的一侧形成一个臂和一个三螺旋DNA结合结构域。这些臂环绕着中央16碱基对的小沟,DNA结合结构域与结合位点外边界附近的大沟相互作用。解离酶二聚体是不对称的,特别是在臂区域,这意味着一种构象适应性,这可能对解离酶结合突触体中不同的DNA位点很重要。这也增加了顺序单链切割机制的可能性。

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