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TodT反应调节因子与其在tod途径操纵子启动子处的多个识别位点的分层结合。

Hierarchical binding of the TodT response regulator to its multiple recognition sites at the tod pathway operon promoter.

作者信息

Lacal Jesús, Guazzaroni María Eugenia, Busch Andreas, Krell Tino, Ramos Juan L

机构信息

Department of Environmental Protection, Estación Experimental del Zaidín, Consejo Superior de Investigaciones Científicas, Calle Profesor Albareda, 1, E-18008 Granada, Spain.

出版信息

J Mol Biol. 2008 Feb 15;376(2):325-37. doi: 10.1016/j.jmb.2007.12.004. Epub 2007 Dec 8.

DOI:10.1016/j.jmb.2007.12.004
PMID:18166197
Abstract

The TodS and TodT proteins form a highly specific two-component regulatory system that controls the expression of genes involved in the degradation of toluene, benzene, and ethylbenzene via the toluene dioxygenase pathway. The catabolic genes of the toluene dioxygenase pathway are transcribed from a single promoter called P(todX) once the response regulator TodT is phosphorylated by the TodS sensor kinase in response to pathway substrates. We show here that TodT is a monomer in solution and that it binds to three specific sites in the P(todX) promoter, centered at -57, -85, and -106 with respect to the transcription start site. The -85 and -106 sites are pseudopalindromic, whereas the -57 site is half a palindrome. TodT binding to its target sites is sequential, as shown by electrophoresis mobility gel shift assays and footprinting. The binding affinity values of TodT, as determined by isothermal titration calorimetry, are 1.8+/-0.2, 5+/-0.4, and 6.3+/-0.8 microM for the -106, -85, and -57 sites, respectively, and the binding stoichiometry is one monomer per half-palindromic element. Mutational analysis revealed that all three sites contribute to P(todX) strength, although the most relevant site is the distal one with respect to the -10 extended element of the downstream promoter element. The C-TodT [C-terminal TodT fragment (amino acids 154-206)], a truncated variant of TodT that contains the C-terminal half of the protein bearing the DNA binding domain, binds in vitro to all three sites with affinity similar to that of the full-length protein. However, C-TodT, in contrast to the full-length regulator, does not activate in vitro transcription from P(todX). We discuss the consequences of the organization of the binding sites on transcriptional control and propose that the N-terminal domain of TodT is necessary for appropriate interactions with other transcriptional elements.

摘要

TodS和TodT蛋白形成一个高度特异性的双组分调节系统,该系统通过甲苯双加氧酶途径控制参与甲苯、苯和乙苯降解的基因的表达。一旦响应调节因子TodT被TodS传感器激酶磷酸化以响应途径底物,甲苯双加氧酶途径的分解代谢基因就从一个名为P(todX)的单一启动子转录。我们在此表明,TodT在溶液中是单体,并且它与P(todX)启动子中的三个特定位点结合,相对于转录起始位点,这些位点分别位于-57、-85和-106处。-85和-106位点是假回文序列,而-57位点是半回文序列。如电泳迁移率凝胶迁移分析和足迹分析所示,TodT与其靶位点的结合是顺序性的。通过等温滴定量热法测定,TodT对-106、-85和-57位点的结合亲和力值分别为1.8±0.2、5±0.4和6.3±0.8 μM,结合化学计量为每个半回文元件一个单体。突变分析表明,所有三个位点都对P(todX)的强度有贡献,尽管最相关的位点是相对于下游启动子元件的-10延伸元件的远端位点。C-TodT [TodT C端片段(氨基酸154 - 206)]是TodT的截短变体,包含带有DNA结合结构域的蛋白质的C端一半,它在体外与所有三个位点结合,亲和力与全长蛋白质相似。然而,与全长调节因子相反,C-TodT不能在体外激活P(todX)的转录。我们讨论了结合位点的组织对转录控制的影响,并提出TodT的N端结构域对于与其他转录元件进行适当相互作用是必需的。

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