The glutamate effect on DNA binding by pol I DNA polymerases: osmotic stress and the effective reversal of salt linkage.

Deredge DJ; Baker JT; Datta K; Licata VJ

首页> 外文期刊>Journal of Molecular Biology >The glutamate effect on DNA binding by pol I DNA polymerases: osmotic stress and the effective reversal of salt linkage.

【24h】

The glutamate effect on DNA binding by pol I DNA polymerases: osmotic stress and the effective reversal of salt linkage.

机译：谷氨酸对pol I DNA聚合酶与DNA结合的影响：渗透胁迫和盐键的有效逆转。

获取原文

获取原文并翻译 | 示例

获取外文期刊封面封底 >>

开具论文收录证明 >>

文献代查 >>

团队文献服务 >>

页面导航

摘要
著录项
引文网络
相似文献
相关主题

摘要

The significant enhancing effect of glutamate on DNA binding by Escherichia coli nucleic acid binding proteins has been extensively documented. Glutamate has also often been observed to reduce the apparent linked ion release (Deltan(ions)) upon DNA binding. In this study, it is shown that the Klenow and Klentaq large fragments of the Type I DNA polymerases from E. coli and Thermus aquaticus both display enhanced DNA binding affinity in the presence of glutamate versus chloride. Across the relatively narrow salt concentration ranges often used to obtain salt linkage data, Klenow displays an apparently decreased Deltan(ions) in the presence of Kglutamate, while Klentaq appears not to display an anion-specific effect on Deltan(ions). Osmotic stress experiments reveal that DNA binding by Klenow and Klentaq is associated with the release of approximately 500 to 600 waters in the presence of KCl. For both proteins, replacing chloride with glutamate results in a 70% reduction in the osmotic-stress-measured hydration change associated with DNA binding (to approximately 150-200 waters released), suggesting that glutamate plays a significant osmotic role. Measurements of the salt-DNA binding linkages were extended up to 2.5 M Kglutamate to further examine this osmotic effect of glutamate, and it is observed that a reversal of the salt linkage occurs above 800 mM for both Klenow and Klentaq. Salt-addition titrations confirm that an increase of [Kglutamate] beyond 1 M results in rebinding of salt-displaced polymerase to DNA. These data represent a rare documentation of a reversed ion linkage for a protein-DNA interaction (i.e., enhanced binding as salt concentration increases). Nonlinear linkage analysis indicates that this unusual behavior can be quantitatively accounted for by a shifting balance of ionic and osmotic effects as [Kglutamate] is increased. These results are predicted to be general for protein-DNA interactions in glutamate salts.

机译：谷氨酸对大肠杆菌核酸结合蛋白与DNA结合的显着增强作用已被广泛记录。还经常观察到谷氨酸在DNA结合后减少表观的连接离子释放（Deltan（离子））。在这项研究中，表明在谷氨酸对氯化物存在下，大肠杆菌和水生栖热菌的I型DNA聚合酶的Klenow和Klentaq大片段都显示出增强的DNA结合亲和力。在通常用于获得盐键数据的相对较窄的盐浓度范围内，Klenow在存在谷氨酸盐的情况下显示出明显降低的Deltan（离子），而Klentaq似乎对Deltan（离子）没有显示出阴离子特异性作用。渗透胁迫实验表明，在存在KCl的情况下，Klenow和Klentaq的DNA结合与大约500至600水的释放有关。对于这两种蛋白质，用谷氨酸代替氯化物可导致与DNA结合相关的渗透压测量水化变化降低70％（释放到约150-200个水），这表明谷氨酸发挥了重要的渗透作用。盐-DNA结合键的测量扩展到2.5 M Kglutamate，以进一步检查谷氨酸的这种渗透作用，并且观察到Klenow和Klentaq在800 mM以上都发生了盐键的逆转。盐滴定法证实[Kglutamate]的增加超过1 M会导致盐置换的聚合酶与DNA重新结合。这些数据代表了蛋白质-DNA相互作用的反向离子键的稀有文献（即，随着盐浓度的增加，结合增强）。非线性连锁分析表明，随着[Kglutamate]的增加，这种异常行为可以通过离子和渗透作用的移动平衡来定量解决。预测这些结果对于谷氨酸盐中的蛋白质-DNA相互作用是通用的。

著录项

来源
《Journal of Molecular Biology》 |2010年第2期|共16页
作者
Deredge DJ; Baker JT; Datta K; Licata VJ;
展开▼
作者单位

展开▼
收录信息
原文格式 PDF
正文语种 eng
中图分类
关键词

相似文献

外文文献
中文文献
专利

1. The glutamate effect on DNA binding by pol I DNA polymerases: osmotic stress and the effective reversal of salt linkage. [J] . Deredge DJ, Baker JT, Datta K, Journal of Molecular Biology . 2010,第2期

机译：谷氨酸对pol I DNA聚合酶与DNA结合的影响：渗透胁迫和盐键的有效逆转。
2. Probing DNA Binding, DNA Opening, and Assembly of a Downstream Clamp/Jaw in Escherichia coli RNA Polymerase−λPR Promoter Complexes Using Salt and the Physiological Anion Glutamate [J] . Wayne S. Kontur Michael W. Capp Theodore J. Gries Ruth M. Saecker and M. Thomas Record Jr. Biochemistry . 2010,第20期

机译：使用盐和生理性谷氨酸负离子探测大肠杆菌RNA聚合酶-λPR启动子复合物中DNA的结合，DNA的开放和组装。
3. Probing DNA binding, DNA opening, and assembly of a downstream clamp/jaw in escherichia coli RNA polymerase-λPR promoter complexes using salt and the physiological anion glutamate [J] . Kontur W.S., Capp M.W., Gries T.J., Biochemistry . 2010,第20期

机译：使用盐和生理性谷氨酸阴离子探测大肠杆菌RNA聚合酶-λPR启动子复合物中的DNA结合，DNA打开和下游钳夹/钳口的组装
4. Towards an understanding of protein-protein interaction network hierarchies. Analysis of DnaN (β)-binding peptide motifs in members of protein families interacting with the eubacterial processivity clamp, the β subunit of DNA Polymerase III [C] . Brian P. Dalrymple, Gene Wijffels, Kritaya Kongsuwan, Asia-Pacific Bioinformatics Conference(APBC 2003); 200302; Adelaide(AU) . 2003

机译：对蛋白质-蛋白质相互作用网络层次结构的理解。蛋白质家族成员与DNA聚合酶III的优生过程性钳位相互作用的DnaN（β）结合肽基序分析
5. Electronic control of DNA polymerase binding and unbinding to single DNA molecules tethered in a nanopore. [D] . Wilson, Noah A. 2009

机译：电子控制DNA聚合酶与纳米孔中束缚的单个DNA分子结合和不结合。
6. Probing DNA Binding DNA Opening and Assembly of a Downstream Clamp/Jaw in E. coli RNA Polymerase – λPR Promoter Complexes Using Salt and the Physiological Anion Glutamate [O] . Wayne S. Kontur, Michael W. Capp, Theodore J. Gries, -1

机译：探测DNa结合一个下游夹紧装置/颚在大肠杆菌RNa聚合酶的DNa打开和装配 - λpR启动子配合物使用盐和生理阴离子谷氨酸
7. Probing DNA Binding, DNA Opening, and Assembly of a Downstream Clamp/Jaw in Escherichia coli RNA Polymerase−λPR Promoter Complexes Using Salt and the Physiological Anion Glutamate [O] . Wayne S. Kontur, Michael W. Capp, Theodore J. Gries, 2010

机译：使用盐和生理阴离子谷氨酸的大肠杆菌RNA聚合酶-λpr启动子复合物中下游夹具/钳口的DNA结合，DNA开口和组装

The glutamate effect on DNA binding by pol I DNA polymerases: osmotic stress and the effective reversal of salt linkage.

摘要

著录项

引文网络

相似文献

相关主题

期刊订阅