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DNA 中的单个错配会诱导 MutS 的聚集增强。蛋白质-DNA 复合物的流体动力学分析。

A single mismatch in the DNA induces enhanced aggregation of MutS. Hydrodynamic analyses of the protein-DNA complexes.

作者信息

Nag Nabanita, Krishnamoorthy G, Rao Basuthkar J

机构信息

Department of Chemical Sciences, Tata Institute of Fundamental Research, Mumbai, India.

出版信息

FEBS J. 2005 Dec;272(24):6228-43. doi: 10.1111/j.1742-4658.2005.04997.x.

Abstract

Changes in the oligomeric status of MutS protein was probed in solution by dynamic light scattering (DLS), and corroborated by sedimentation analyses. In the absence of any nucleotide cofactor, free MutS protein [hydrodynamic radius (Rh) of 10-12 nm] shows a small increment in size (Rh 14 nm) following the addition of homoduplex DNA (121 bp), whereas the same increases to about 18-20 nm with heteroduplex DNA containing a mismatch. MutS forms large aggregates (Rh > 500 nm) with ATP, but not in the presence of a poorly hydrolysable analogue of ATP (ATPgammaS). Addition of either homo- or heteroduplex DNA attenuates the same, due to protein recruitment to DNA. However, the same protein/DNA complexes, at high concentration of ATP (10 mm), manifest an interesting property where the presence of a single mismatch provokes a much larger oligomerization of MutS on DNA (Rh > 500 nm in the presence of MutL) as compared to the normal homoduplex (Rh approximately 100-200 nm) and such mismatch induced MutS aggregation is entirely sustained by the ongoing hydrolysis of ATP in the reaction. We speculate that the surprising property of a single mismatch, in nucleating a massive aggregation of MutS encompassing the bound DNA might play an important role in mismatch repair system.

摘要

通过动态光散射(DLS)在溶液中探测MutS蛋白寡聚状态的变化,并通过沉降分析进行验证。在不存在任何核苷酸辅因子的情况下,游离的MutS蛋白[流体动力学半径(Rh)为10 - 12纳米]在加入同型双链DNA(121碱基对)后,大小略有增加(Rh为14纳米),而对于含有错配的异型双链DNA,其大小增加到约18 - 20纳米。MutS与ATP形成大聚集体(Rh > 500纳米),但在存在ATP的难水解类似物(ATPγS)时则不会。加入同型或异型双链DNA会减弱这种情况,这是由于蛋白质被招募到DNA上。然而,在高浓度ATP(10毫米)下,相同的蛋白质/DNA复合物表现出一种有趣的特性,即与正常同型双链(Rh约为100 - 200纳米)相比,单个错配的存在会引发MutS在DNA上更大程度的寡聚化(在MutL存在下Rh > 500纳米),并且这种错配诱导的MutS聚集完全由反应中ATP的持续水解维持。我们推测,单个错配在引发包含结合DNA的MutS大量聚集方面的惊人特性可能在错配修复系统中起重要作用。

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