Salt Modulates Oligomerization Properties of hRad51 and hRad52 Proteins

Kamakshi Balakrishnan, N. Krishnan, B. Rao
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引用次数: 1

Abstract

Human Rad52 (hRad52) and Rad51 (hRad51) proteins are important components of homologous recombination machinery involved in DNA double strand break repair. hRad52 subunits oligomerize to form rings, which are further believed to stack one over another giving rise to higher order structures. Such structures bind the ends of duplex DNA to bring about DNA end joining. hRad51 exists in the native state as oligomeric rings and monomerizes to interact with the DNA. In our current study, we report disruption and solubilization of hRad52 aggregates and higher order aggregation of hRad51 molecules at high salt (KCl) concentration. Computational analysis of the crystal structure available for N-terminal 212 amino acids of hRad52 protein reveal a dense unique distribution of salt bridges, not only between adjacent but also between penultimate subunit neighbors which perhaps contribute to stabilization of hRad52 oligomeric rings. Our results suggest that disruption of inter-subunit salt bridges and thereby perturbation of interaction between individual monomers as the underlying mechanism for salt mediated monomerization of hRad52 protein. The crystal structure of Rad51 on the other hand lacks such dense salt-bridge connectivity suggesting that salt-mediated monomerization is a feature of proteins with dense salt-bridge networks. Salt brings together the hydrophobic surface residues of hRad51 in a process termed as "salting out" resulting in aggregation of hRad51 molecules. Given the functional relevance of oligomeric hRad52 and monomeric hRad51 in homologous recombination mediated repair, our findings imply that salt regulates the oligomerization status of these repair proteins, and thereby, their functions respectively.
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盐调节hRad51和hRad52蛋白的寡聚化特性
人类Rad52 (hRad52)和Rad51 (hRad51)蛋白是参与DNA双链断裂修复的同源重组机制的重要组成部分。hRad52亚基寡聚形成环,进一步认为这些环可以堆叠在一起,从而产生更高阶的结构。这种结构结合双链DNA的末端,导致DNA末端连接。hRad51在天然状态下以寡聚环的形式存在,并单体化与DNA相互作用。在我们目前的研究中,我们报告了高盐(KCl)浓度下hRad52聚集体的破坏和溶解以及hRad51分子的高阶聚集。对hRad52蛋白n端212个氨基酸晶体结构的计算分析表明,不仅在相邻亚基之间,而且在倒数第二亚基邻居之间,盐桥分布密集,这可能有助于hRad52寡聚环的稳定。我们的研究结果表明,亚基间盐桥的破坏和单个单体之间相互作用的扰动是盐介导hRad52蛋白单体化的潜在机制。另一方面,Rad51的晶体结构缺乏这种密集的盐桥连通性,这表明盐介导的单体化是具有密集盐桥网络的蛋白质的一个特征。盐将hRad51的疏水表面残基聚集在一起,这一过程被称为“盐析”,导致hRad51分子聚集。鉴于低聚体hRad52和单体hRad51在同源重组介导的修复中的功能相关性,我们的研究结果表明,盐调节了这些修复蛋白的低聚状态,从而分别调节了它们的功能。
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