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The Structures of T87I Phosphono-CheY and T87I/Y106W Phosphono-CheY Help to Explain Their Binding Affinities to the FliM and CheZ Peptides

机译:T87I Phosphono-CheY和T87I / Y106W Phosphono-CheY的结构有助于说明它们与FliM和CheZ肽的结合亲和力

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摘要

CheY is a response regulator in bacterial chemotaxis. E. coli CheY mutants T87I and T87I/Y106W CheY are phosphorylatable on Asp57 but unable to generate clockwise rotation of the flagella. To understand this phenotype in terms of structure, stable analogs of the two CheY-P mutants were synthesized: T87I phosphono-CheY and T87I phosphono-CheY. Dissociation constants for peptides derived from flagellar motor protein FliM and phosphatase CheZ were determined for phosphono-CheY and the two mutants. The peptides bind phosphono-CheY almost as strongly as CheY-P; however, they do not bind T87I phosphono-CheY or T87I/Y106W phosphono-CheY, implying that the mutant proteins cannot bind FliM or CheZ tightly in vivo. The structures of T87I phosphono-CheY and T87I/Y106W phosphono-CheY were solved to resolutions of 1.8 Å and 2.4 Å, respectively. The increased bulk of I87 forces the side chain of Y106 or W106, into a more solvent-accessible conformation, which occludes the peptide-binding site.
机译:CheY是细菌趋化性的响应调节剂。大肠杆菌CheY突变体T87I和T87I / Y106W CheY在Asp57上可磷酸化,但无法产生鞭毛的顺时针旋转。为了从结构上理解该表型,合成了两个CheY-P突变体的稳定类似物:T87I膦酰基-CheY和T87I膦酰基-CheY。测定了膦酰-CheY和两个突变体的衍生自鞭毛运动蛋白FliM和磷酸酶CheZ的肽的解离常数。肽结合膦酰-CheY的强度几乎与CheY-P相同。但是,它们不结合T87I膦酰基-CheY或T87I / Y106W膦酰基-CheY,这意味着突变蛋白不能在体内紧密结合FliM或CheZ。 T87I膦酰基-CheY和T87I / Y106W膦酰基-CheY的结构分别解析为1.8Å和2.4Å的分辨率。 I87的增加的体积迫使Y106或W106的侧链变成更易接近溶剂的构象,从而使肽结合位点闭塞。

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