大肠杆菌的类管蛋白 FtsZ 的结构域间隙中的盐桥相互作用被破坏,使细胞对细胞分裂抑制剂 PC190723 敏感。

Sakshi Mahesh Poddar, Joyeeta Chakraborty, Pananghat Gayathri, Ramanujam Srinivasan
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引用次数: 0

摘要

FtsZ 在细菌分裂部位形成环状集合体。它是第一个参与形成分裂体复合物的蛋白质,将细胞分成两半,这表明它在细菌细胞分裂中的重要性。FtsZ 是开发新型抗微生物药物以克服抗生素耐药性挑战的一个极具吸引力的靶点。对 FtsZ 最有效的抑制剂是 PC190723,它对所有葡萄球菌菌株和菌种都有效,包括耐甲氧西林和耐多种药物的金黄色葡萄球菌和芽孢杆菌菌株。然而,大肠杆菌、链球菌和肠球菌等细菌的 FtsZs 对这种抑制剂具有抗药性。在本研究中,我们提供了进一步的证据,证明在 S7、S9、S10 β 链和 H7 螺旋之间的残基 S227 和 G191、R307 和 E198 以及 D299 和 R202 之间的三对桥接相互作用阻止了抑制剂与大肠杆菌 FtsZ 的结合。我们产生了单突变、双突变和三突变来破坏这些桥,并测试了 PC190723 直接在体内对 Z 环组装的有效性。结果表明,S227-G191 和 R307-E198 桥的破坏使 EcFtsZ 对 PC190723 的 Z 环组装高度敏感。异位表达双突变体 FtsZ S227I R307V 会导致易感的大肠杆菌 imp4213 菌株对 PC190723 超敏。我们的研究可以进一步预测 PC190723 或其衍生物对其他细菌属的 FtsZ 的有效性。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Disruption of salt bridge interactions in the inter-domain cleft of the tubulin-like protein FtsZ of Escherichia coli makes cells sensitive to the cell division inhibitor PC190723.

FtsZ forms a ring-like assembly at the site of division in bacteria. It is the first protein involved in the formation of the divisome complex to split the cell into two halves, indicating its importance in bacterial cell division. FtsZ is an attractive target for developing new anti-microbial drugs to overcome the challenges of antibiotic resistance. The most potent inhibitor against FtsZ is PC190723, which is effective against all strains and species of Staphylococcus, including the methicillin- and multi-drug-resistant Staphylococcus aureus and strains of Bacillus. However, FtsZs from bacteria such as E. coli, Streptococcus, and Enterococcus were shown to be resistant to this inhibitor. In this study, we provide further evidence that the three pairwise bridging interactions, between residues S227 and G191, R307 and E198 and D299 and R202, between S7, S9, S10 β-strands and the H7 helix occlude the inhibitor from binding to E. coli FtsZ. We generated single, double and triple mutations to disrupt those bridges and tested the effectiveness of PC190723 directly on Z-ring assembly in vivo. Our results show that the disruption of S227-G191 and R307-E198 bridges render EcFtsZ highly sensitive to PC190723 for Z-ring assembly. Ectopic expression of the double mutants, FtsZ S227I R307V results in hypersensitivity of the susceptible E. coli imp4213 strain to PC190723. Our studies could further predict the effectiveness of PC190723 or its derivatives towards FtsZs of other bacterial genera.

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