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指导解离酶位点特异性重组的蛋白质-蛋白质相互作用:结构-功能分析

Protein-protein interactions directing resolvase site-specific recombination: a structure-function analysis.

作者信息

Hughes R E, Rice P A, Steitz T A, Grindley N D

机构信息

Department of Molecular Biophysics and Biochemistry, Yale University, New Haven, CT 06510.

出版信息

EMBO J. 1993 Apr;12(4):1447-58. doi: 10.1002/j.1460-2075.1993.tb05788.x.

Abstract

Recombination catalyzed by the gamma delta resolvase requires assembly of a nucleo-protein complex, the synaptosome, whose structure is determined by resolvase-res and resolvase-resolvase interactions. In crystals of the resolvase catalytic domain, monomers of resolvase were closely associated with one another across three different dyad axes; one of these subunit contacts was shown to be an essential inter-dimer interaction. To investigate the relevance of the remaining two interfaces, we have made site-directed mutations at positions suggested by the structure. Cysteine substitutions were designed to link the interfaces covalently, mutations to arginine were used to disrupt intersubunit contacts, and mutations to tryptophan were used to study the hydrophobicity and solvent accessibility of potential interfaces by fluorescence quenching. Characterization of the mutant proteins has allowed us to identify the dimer interface of resolvase and to assign a structural role to a second intersubunit contact. The data presented here, together with our previous results, suggest that all three of the dyad-related intersubunit interactions observed in the crystal play specific roles in synapsis and recombination.

摘要

由γδ解离酶催化的重组反应需要一种核蛋白复合物——联会体的组装,其结构由解离酶 - res以及解离酶 - 解离酶之间的相互作用所决定。在解离酶催化结构域的晶体中,解离酶单体在三个不同的二重对称轴上彼此紧密相连;其中一种亚基接触被证明是一种必不可少的二聚体间相互作用。为了研究其余两个界面的相关性,我们在结构所提示的位置进行了定点突变。半胱氨酸取代旨在共价连接界面,突变为精氨酸用于破坏亚基间接触,突变为色氨酸则用于通过荧光猝灭研究潜在界面的疏水性和溶剂可及性。对突变蛋白的表征使我们能够确定解离酶的二聚体界面,并为另一种亚基间接触赋予结构作用。此处呈现的数据,连同我们之前的结果表明,在晶体中观察到的所有三种与二重轴相关的亚基间相互作用在联会和重组中都发挥着特定作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7529/413356/6a5af3189f9c/emboj00076-0192-a.jpg

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