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Single-molecule analysis reveals two separate DNA-binding domains in the Escherichia coli UvrA dimer

机译:单分子分析揭示了大肠杆菌UvrA二聚体中的两个独立的DNA结合域

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摘要

The UvrA protein is the initial damage-recognizing factor in bacterial nucleotide excision repair. Each monomer of the UvrA dimer contains two ATPase sites. Using single-molecule analysis we show that dimerization of UvrA in the presence of ATP is significantly higher than with ADP or nonhydrolyzable ATPγS, suggesting that the active UvrA dimer contains a mixture of ADP and ATP. We also show that the UvrA dimer has a high preference of binding the end of a linear DNA fragment, independent on the presence or type of cofactor. Apparently ATP binding or hydrolysis is not needed to discriminate between DNA ends and internal sites. A significant number of complexes could be detected where one UvrA dimer bridges two DNA ends implying the presence of two separate DNA-binding domains, most likely present in each monomer. On DNA containing a site-specific lesion the damage-specific binding is much higher than DNA-end binding, but only in the absence of cofactor or with ATP. With ATPγS no discrimination between a DNA end and a DNA damage could be observed. We present a model where damage recognition of UvrA depends on the ability of both UvrA monomers to interact with the DNA flanking the lesion.
机译:UvrA蛋白是细菌核苷酸切除修复中的初始损伤识别因子。 UvrA二聚体的每个单体均包含两个ATPase位点。使用单分子分析,我们发现在ATP存在下UvrA的二聚化显着高于ADP或不可水解的ATPγS,表明活性UvrA二聚体包含ADP和ATP的混合物。我们还显示,UvrA二聚体具有高度的优先权,可以结合线性DNA片段的末端,而与辅因子的存在或类型无关。显然,不需要ATP结合或水解来区分DNA末端和内部位点。可以检测到大量复合物,其中一个UvrA二聚体桥接两个DNA末端,表明存在两个单独的DNA结合域,每个单体中最有可能存在。在含有位点特异性病变的DNA上,损伤特异性结合远高于DNA末端结合,但仅在不存在辅因子或与ATP结合的情况下。使用ATPγS不能观察到DNA末端和DNA损伤之间的区别。我们提出了一个模型,其中UvrA的损伤识别取决于两个UvrA单体与病变两侧的DNA相互作用的能力。

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