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Structural Insights into Substrate Recognition by Clostridium difficile Sortase

机译:难辨梭状芽孢杆菌分选酶对底物识别的结构见解。

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摘要

Sortases function as cysteine transpeptidases that catalyze the covalent attachment of virulence-associated surface proteins into the cell wall peptidoglycan in Gram-positive bacteria. The substrate proteins targeted by sortase enzymes have a cell wall sorting signal (CWSS) located at the C-terminus. Up to date, it is still not well understood how sortases with structural resemblance among different classes and diverse species of bacteria achieve substrate specificity. In this study, we focus on elucidating the molecular basis for specific recognition of peptide substrate PPKTG by Clostridium difficile sortase B (Cd-SrtB). Combining structural studies, biochemical assays and molecular dynamics simulations, we have constructed a computational model of Cd-SrtBΔN26–PPKTG complex and have validated the model by site-directed mutagensis studies and fluorescence resonance energy transfer (FRET)-based assay. Furthermore, we have revealed that the fourth amino acid in the N-terminal direction from cleavage site of PPKTG forms specific interaction with Cd-SrtB and plays an essential role in configuring the peptide to allow more efficient substrate-specific cleavage by Cd-SrtB.
机译:分选酶起半胱氨酸转肽酶的作用,可催化与毒性相关的表面蛋白与革兰氏阳性细菌的细胞壁肽聚糖共价结合。分选酶靶向的底物蛋白具有位于C端的细胞壁分选信号(CWSS)。迄今为止,仍不完全了解在不同类别和不同种类的细菌之间具有结构相似性的分选酶如何实现底物特异性。在这项研究中,我们专注于阐明艰难梭菌分选酶B(Cd-SrtB)特异性识别肽底物PPKTG的分子基础。结合结构研究,生化分析和分子动力学模拟,我们构建了Cd-SrtBΔN26-PPKTG复合物的计算模型,并通过定点诱变研究和基于荧光共振能量转移(FRET)的分析验证了该模型。此外,我们已经揭示,从PPKTG的切割位点开始在N末端方向的第四个氨基酸与Cd-SrtB形成特异性相互作用,并且在配置该肽以通过Cd-SrtB进行更有效的底物特异性切割中起着至关重要的作用。

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