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甲基化片段对于大肠杆菌的甲基接受丝氨酸化学感受器Tsr的细胞质片段进行趋化信号传导不是必需的。

Methylation segments are not required for chemotactic signalling by cytoplasmic fragments of Tsr, the methyl-accepting serine chemoreceptor of Escherichia coli.

作者信息

Ames P, Yu Y A, Parkinson J S

机构信息

Biology Department, University of Utah, Salt Lake City 84112, USA.

出版信息

Mol Microbiol. 1996 Feb;19(4):737-46. doi: 10.1046/j.1365-2958.1996.408930.x.

DOI:10.1046/j.1365-2958.1996.408930.x
PMID:8820644
Abstract

The serine chemoreceptor Tsr and other methyl-accepting chemotaxis proteins (MCPs) control the swimming behaviour of Escherichia coli by generating signals that influence the direction of flagellar rotation. MCPs produce clockwise (CW) signals by stimulating the autophosphorylation activity of CheA, a cytoplasmic histidine kinase, and counter-clockwise signals by inhibiting CheA. CheW couples CheA to chemoreceptor control by promoting formation of MCP/CheW/CheA ternary complexes. To identify MCP structural determinants essential for CheA stimulation, we inserted fragments of the tsr coding region into an inducible expression vector and used a swimming contest called 'pseudotaxis' to select for transformant cells carrying CW-signalling plasmids. The shortest active fragment we found, Tsr (350-470), stimulated CheA in a CheW-dependent manner, as full-length Tsr molecules do. It spans a highly conserved 'core' (370-420) that probably specifies the CheA and CheW contact sites and other determinants needed for stimulatory control of CheA. Tsr (350-470) also carries portions of the left and right arms flanking the core, which probably play roles in regulating MCP signalling state. However, this Tsr fragment lacks all of the methylation sites characteristic of MCP molecules, indicating that methylation segments are not essential for generating receptor output signals.

摘要

丝氨酸化学感受器Tsr和其他甲基化接受趋化蛋白(MCPs)通过产生影响鞭毛旋转方向的信号来控制大肠杆菌的游动行为。MCPs通过刺激细胞质组氨酸激酶CheA的自磷酸化活性产生顺时针(CW)信号,并通过抑制CheA产生逆时针信号。CheW通过促进MCP/CheW/CheA三元复合物的形成将CheA与化学感受器控制联系起来。为了确定对CheA刺激至关重要的MCP结构决定因素,我们将tsr编码区的片段插入到一个可诱导表达载体中,并使用一种名为“假趋化”的游动竞赛来筛选携带CW信号质粒的转化细胞。我们发现的最短活性片段Tsr(350-470)以依赖CheW的方式刺激CheA,就像全长Tsr分子一样。它跨越一个高度保守的“核心”区域(370-420),该区域可能确定了CheA和CheW的接触位点以及对CheA进行刺激控制所需的其他决定因素。Tsr(350-470)还带有核心两侧左臂和右臂的部分,这可能在调节MCP信号状态中发挥作用。然而,这个Tsr片段缺乏MCP分子特有的所有甲基化位点,这表明甲基化片段对于产生受体输出信号不是必需的。

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