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多药/脂 A ABC 外排泵 MsbA 的构象循环的解析。

Dissection of the conformational cycle of the multidrug/lipidA ABC exporter MsbA.

机构信息

Department of Pharmacology, University of Cambridge, Cambridge CB2 1PD, United Kingdom.

出版信息

Proteins. 2010 Nov 1;78(14):2867-72. doi: 10.1002/prot.22813.

DOI:10.1002/prot.22813
PMID:20715055
Abstract

Recent crystal structures of the multidrug ATP-binding cassette (ABC) exporters Sav1866 from Staphylococcus aureus, MsbA from Escherichia coli, Vibrio cholera, and Salmonella typhimurium, and mouse ABCB1a suggest a common alternating access mechanism for export. However, the molecular framework underlying this mechanism is critically dependent on assumed conformational relationships between nonidentical crystal structures and therefore requires biochemical verification. The structures of homodimeric MsbA reveal a pair of glutamate residues (E208 and E208') in the intracellular domains of its two half-transporters, close to the nucleotide-binding domains (NBDs), which are in close proximity of each other in the outward-facing state but not in the inward-facing state. Using intermolecular cysteine crosslinking between E208C and E208C' in E. coli MsbA, we demonstrate that the NBDs dissociate in nucleotide-free conditions and come close on ATP binding and ADP·vanadate trapping. Interestingly, ADP alone separates the half-transporters like a nucleotide-free state, presumably for the following catalytic cycle. Our data fill persistent gaps in current studies on the conformational dynamics of a variety of ABC exporters. Based on a single biochemical method, the findings describe a conformational cycle for a single ABC exporter at major checkpoints of the ATPase reaction under experimental conditions, where the exporter is transport active.

摘要

最近的晶体结构研究表明,金黄色葡萄球菌的多药 ATP 结合盒(ABC)外排泵 Sav1866、大肠杆菌的 MsbA、霍乱弧菌和鼠源 ABCB1a 具有共同的交替访问机制,用于外排。然而,这种机制的分子框架严重依赖于假定的非同源晶体结构之间的构象关系,因此需要生化验证。同源二聚体 MsbA 的结构揭示了其两个半转运蛋白细胞内结构域中的一对谷氨酸残基(E208 和 E208'),靠近核苷酸结合域(NBD),在向外开放状态下彼此靠近,但在内向开放状态下不靠近。我们使用大肠杆菌 MsbA 中 E208C 和 E208C'之间的分子间半胱氨酸交联,证明在无核苷酸条件下 NBD 解离,在 ATP 结合和 ADP·钒酸盐捕获时靠近。有趣的是,ADP 单独分离半转运蛋白,就像在无核苷酸状态下一样,可能是为了以下的催化循环。我们的数据填补了当前对各种 ABC 外排泵构象动力学研究中持续存在的空白。基于单一的生化方法,这些发现描述了在实验条件下,在 ATP 酶反应的主要检查点下,一种 ABC 外排泵的构象循环,此时外排泵具有转运活性。

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