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保守组氨酸-243在EnvZ磷酸酶活性中的作用,EnvZ是大肠杆菌中孔蛋白渗透调节的传感器。

Function of conserved histidine-243 in phosphatase activity of EnvZ, the sensor for porin osmoregulation in Escherichia coli.

作者信息

Hsing W, Silhavy T J

机构信息

Department of Molecular Biology, Princeton University, New Jersey 08544, USA.

出版信息

J Bacteriol. 1997 Jun;179(11):3729-35. doi: 10.1128/jb.179.11.3729-3735.1997.

Abstract

EnvZ and OmpR are the sensor and response regulator proteins of a two-component system that controls the porin regulon of Escherichia coli in response to osmolarity. Three enzymatic activities are associated with EnvZ: autokinase, OmpR kinase, and OmpR-phosphate (OmpR-P) phosphatase. Conserved histidine-243 is critical for both autokinase and OmpR kinase activities. To investigate its involvement in OmpR-P phosphatase activity, histidine-243 was mutated to several other amino acids and the phosphatase activity of mutated EnvZ was measured both in vivo and in vitro. In agreement with previous reports, we found that certain substitutions abolished the phosphatase activity of EnvZ. However, a significant level of phosphatase activity remained when histidine-243 was replaced with certain amino acids, such as tyrosine. In addition, the phosphatase activity of a previously identified kinase- phosphatase+ mutant was not abolished by the replacement of histidine-243 with asparagine. These data indicated that although conserved histidine-243 is important for the phosphatase activity, a histidine-243-P intermediate is not required. Our data are consistent with a previous model that proposes a common transition state with histidine-243 (EnvZ) in close contact with aspartate-55 (OmpR) for both OmpR phosphorylation and dephosphorylation. Phosphotransfer occurs from histidine-243-P to aspartate-55 during phosphorylation, but water replaces the phosphorylated histidine side chain leading to hydrolysis during dephosphorylation.

摘要

EnvZ和OmpR是一个双组分系统中的传感蛋白和反应调节蛋白,该系统可根据渗透压控制大肠杆菌的孔蛋白调节子。EnvZ具有三种酶活性:自身激酶、OmpR激酶和OmpR - 磷酸(OmpR - P)磷酸酶。保守的组氨酸 - 243对自身激酶和OmpR激酶活性都至关重要。为了研究其在OmpR - P磷酸酶活性中的作用,将组氨酸 - 243突变为其他几种氨基酸,并在体内和体外测量突变型EnvZ的磷酸酶活性。与之前的报道一致,我们发现某些替代会消除EnvZ的磷酸酶活性。然而,当组氨酸 - 243被某些氨基酸(如酪氨酸)取代时,仍保留了相当水平的磷酸酶活性。此外,用天冬酰胺取代组氨酸 - 243并没有消除先前鉴定的激酶 - 磷酸酶 + 突变体的磷酸酶活性。这些数据表明,虽然保守的组氨酸 - 243对磷酸酶活性很重要,但不需要组氨酸 - 243 - P中间体。我们的数据与之前的模型一致,该模型提出在OmpR磷酸化和去磷酸化过程中,组氨酸 - 243(EnvZ)与天冬氨酸 - 55(OmpR)紧密接触形成共同的过渡态。磷酸转移在磷酸化过程中从组氨酸 - 243 - P转移到天冬氨酸 - 55,但在去磷酸化过程中,水取代了磷酸化的组氨酸侧链导致水解。

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