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木糖葡萄球菌全长HPr激酶/磷酸酶在1.95埃分辨率下的结构:模拟磷酸转移反应的产物/底物

Structure of the full-length HPr kinase/phosphatase from Staphylococcus xylosus at 1.95 A resolution: Mimicking the product/substrate of the phospho transfer reactions.

作者信息

Márquez Jose Antonio, Hasenbein Sonja, Koch Brigitte, Fieulaine Sonia, Nessler Sylvie, Russell Robert B, Hengstenberg Wolfgang, Scheffzek Klaus

机构信息

European Molecular Biology Laboratory, Structural and Computational Biology Programme, Meyerhofstrasse 1, 69117 Heidelberg, Germany.

出版信息

Proc Natl Acad Sci U S A. 2002 Mar 19;99(6):3458-63. doi: 10.1073/pnas.052461499.

DOI:10.1073/pnas.052461499
PMID:11904409
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC122545/
Abstract

The histidine containing phospho carrier protein (HPr) kinase/phosphatase is involved in carbon catabolite repression, mainly in Gram-positive bacteria. It is a bifunctional enzyme that phosphorylates Ser-46-HPr in an ATP-dependent reaction and dephosphorylates P-Ser-46-HPr. X-ray analysis of the full-length crystalline enzyme from Staphylococcus xylosus at a resolution of 1.95 A shows the enzyme to consist of two clearly separated domains that are assembled in a hexameric structure resembling a three-bladed propeller. The N-terminal domain has a betaalphabeta fold similar to a segment from enzyme I of the sugar phosphotransferase system and to the uridyl-binding portion of MurF; it is structurally organized in three dimeric modules exposed to form the propeller blades. Two unexpected phosphate ions associated with highly conserved residues were found in the N-terminal dimeric interface. The C-terminal kinase domain is similar to that of the Lactobacillus casei enzyme and is assembled in six copies to form the compact central hub of the propeller. Beyond previously reported similarity with adenylate kinase, we suggest evolutionary relationship with phosphoenolpyruvate carboxykinase. In addition to a phosphate ion in the phosphate-binding loop of the kinase domain, we have identified a second phosphate-binding site that, by comparison with adenylate kinases, we believe accommodates a product/substrate phosphate, normally covalently linked to Ser-46 of HPr. Thus, we propose that our structure represents a product/substrate mimic of the kinase/phosphatase reaction.

摘要

含组氨酸的磷酸载体蛋白(HPr)激酶/磷酸酶参与碳分解代谢物阻遏,主要存在于革兰氏阳性菌中。它是一种双功能酶,在依赖ATP的反应中使Ser-46-HPr磷酸化,并使P-Ser-46-HPr去磷酸化。对木糖葡萄球菌全长晶体酶进行分辨率为1.95 Å的X射线分析表明,该酶由两个明显分开的结构域组成,这些结构域组装成类似三叶螺旋桨的六聚体结构。N端结构域具有β-α-β折叠,类似于糖磷酸转移酶系统中酶I的一个片段以及MurF的尿苷结合部分;它在结构上由三个暴露的二聚体模块组成,形成螺旋桨叶片。在N端二聚体界面发现了两个与高度保守残基相关的意外磷酸根离子。C端激酶结构域与干酪乳杆菌酶的结构域相似,由六个拷贝组装形成螺旋桨紧凑的中心枢纽。除了先前报道的与腺苷酸激酶的相似性外,我们还提出了与磷酸烯醇丙酮酸羧激酶的进化关系。除了激酶结构域磷酸结合环中的一个磷酸根离子外,我们还确定了第二个磷酸结合位点,通过与腺苷酸激酶比较,我们认为该位点容纳一个产物/底物磷酸根,通常与HPr的Ser-46共价连接。因此,我们提出我们的结构代表了激酶/磷酸酶反应的产物/底物模拟物。

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Solution structure of the 40,000 Mr phosphoryl transfer complex between the N-terminal domain of enzyme I and HPr.酶 I 的 N 端结构域与 HPr 之间 40,000 道尔顿磷酰转移复合物的溶液结构
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