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新型苜蓿中华根瘤菌趋化蛋白 CheT 在信号终止和适应中的双重作用。

The dual role of a novel Sinorhizobium meliloti chemotaxis protein CheT in signal termination and adaptation.

机构信息

Department of Biological Sciences, Life Sciences I, Virginia Tech, Blacksburg, Virginia, USA.

Department of Biochemistry and Molecular Biology, Robert Wood Johnson Medical School, Rutgers University, Piscataway, New Jersey, USA.

出版信息

Mol Microbiol. 2024 Oct;122(4):429-446. doi: 10.1111/mmi.15303. Epub 2024 Jul 30.

DOI:10.1111/mmi.15303
PMID:39081077
Abstract

Sinorhizobium meliloti senses nutrients and compounds exuded from alfalfa host roots and coordinates an excitation, termination, and adaptation pathway during chemotaxis. We investigated the role of the novel S. meliloti chemotaxis protein CheT. While CheT and the Escherichia coli phosphatase CheZ share little sequence homology, CheT is predicted to possess an α-helix with a DXXXQ phosphatase motif. Phosphorylation assays demonstrated that CheT dephosphorylates the phosphate-sink response regulator, CheY1P by enhancing its decay two-fold but does not affect the motor response regulator CheY2P. Isothermal Titration Calorimetry (ITC) experiments revealed that CheT binds to a phosphomimic of CheY1P with a K of 2.9 μM, which is 25-fold stronger than its binding to CheY1. Dissimilar chemotaxis phenotypes of the ΔcheT mutant and cheT DXXXQ phosphatase mutants led to the hypothesis that CheT exerts additional function(s). A screen for potential binding partners of CheT revealed that it forms a complex with the methyltransferase CheR. ITC experiments confirmed CheT/CheR binding with a K of 19 μM, and a SEC-MALS analysis determined a 1:1 and 2:1 CheT/CheR complex formation. Although they did not affect each other's enzymatic activity, CheT binding to CheY1P and CheR may serve as a link between signal termination and sensory adaptation.

摘要

苜蓿中华根瘤菌感知紫花苜蓿宿主根系分泌的营养物质和化合物,并在趋化作用过程中协调激发、终止和适应途径。我们研究了新型苜蓿中华根瘤菌趋化性蛋白 CheT 的作用。虽然 CheT 和大肠杆菌磷酸酶 CheZ 序列同源性很小,但 CheT 预测具有一个带有 DXXXQ 磷酸酶基序的α-螺旋。磷酸化实验表明,CheT 通过增强 CheY1P 的衰减来使 CheY1P 去磷酸化,使其衰减增加两倍,但不影响运动响应调节剂 CheY2P。等温滴定量热法(ITC)实验表明,CheT 与 CheY1P 的磷酸模拟物结合的 K 值为 2.9 μM,比与 CheY1 的结合强 25 倍。ΔcheT 突变体和 cheT DXXXQ 磷酸酶突变体的趋化性表型不同,导致假设 CheT 发挥了额外的功能。CheT 潜在结合伙伴的筛选表明,它与甲基转移酶 CheR 形成复合物。ITC 实验证实了 CheT/CheR 结合,K 值为 19 μM,SEC-MALS 分析确定了 1:1 和 2:1 的 CheT/CheR 复合物形成。尽管它们彼此的酶活性没有影响,但 CheT 与 CheY1~P 和 CheR 的结合可能是信号终止和感觉适应之间的联系。

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