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供体链交换和大肠杆菌菌毛形成过程中的构象变化。

Donor strand exchange and conformational changes during E. coli fimbrial formation.

机构信息

Department of Biological Structure, University of Washington, Box 357420, Seattle, WA 98195-7420, USA.

出版信息

J Struct Biol. 2010 Dec;172(3):380-8. doi: 10.1016/j.jsb.2010.06.002. Epub 2010 Jun 4.

DOI:10.1016/j.jsb.2010.06.002
PMID:20570733
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2964381/
Abstract

Fimbriae and pili are macromolecular structures on the surface of Gram negative bacteria that are important for cellular adhesion. A 2.7Å resolution crystal structure of a complex of Escherichia coli fimbrial proteins containing FimH, FimG, FimF, and FimC provides the most complete model to date for the arrangement of subunits assembled in the native structure. The first three proteins form the tip of the fimbriae while FimC is the chaperone protein involved in the usher/chaperone assembly process. The subunits interact through donor strand complementation where a β-strand from a subunit completes the β-sandwich structure of the neighboring subunit or domain closer to the tip of the fimbria. The function of FimC is to provide a surrogate donor strand before delivery of each subunit to the FimD usher and the growing fimbria. Comparison of the subunits in this structure and their chaperone-bound complexes show that the two FimH domains change their relative orientation and position in forming the tip structure. Also, the non-chaperone subunits undergo a conformational change in their first β-strand when the chaperone is replaced by the native donor strand. Some residues move as much as 14Å in the process. This structural shift has not been noted in structural studies of other bacterial adhesion sub-structures assembled via donor strand complementation. The domains undergo a significant structural change in the donor strand binding groove during fimbrial assembly, and this likely plays a role in determining the specificity of subunit-subunit interactions among the fimbrial proteins.

摘要

菌毛和纤毛是革兰氏阴性菌表面的高分子结构,对于细胞黏附非常重要。含有 FimH、FimG、FimF 和 FimC 的大肠杆菌菌毛蛋白复合物的 2.7Å 分辨率晶体结构为天然结构中组装亚基的排列提供了迄今为止最完整的模型。前三种蛋白质形成菌毛的尖端,而 FimC 是参与 usher/chaperone 组装过程的伴侣蛋白。亚基通过供体链互补相互作用,一个亚基的 β-链完成靠近菌毛尖端的相邻亚基或结构域的 β-三明治结构。FimC 的功能是在将每个亚基递送至 FimD usher 和正在生长的菌毛之前,提供替代供体链。比较该结构中的亚基及其伴侣蛋白结合复合物表明,两个 FimH 结构域在形成尖端结构时改变了它们的相对取向和位置。此外,当伴侣蛋白被天然供体链取代时,非伴侣蛋白的第一个 β-链发生构象变化。在此过程中,一些残基移动多达 14Å。在通过供体链互补组装的其他细菌粘附亚结构的结构研究中,没有注意到这种结构移位。在菌毛组装过程中,供体链结合槽中的结构域发生显著的结构变化,这可能在确定菌毛蛋白中亚基-亚基相互作用的特异性方面发挥作用。

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