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通过冷冻电镜研究细胞内囊泡运输和膜重塑。

Probing intracellular vesicle trafficking and membrane remodelling by cryo-EM.

机构信息

Department of Chemistry and Biochemistry, Florida State University, United States.

Department of Biological Sciences, Florida State University, United States; Institute of Molecular Biophysics, Florida State University, United States.

出版信息

J Struct Biol. 2022 Mar;214(1):107836. doi: 10.1016/j.jsb.2022.107836. Epub 2022 Jan 31.

Abstract

Protein transport between the membranous compartments of the eukaryotic cells is mediated by the constant fission and fusion of the membrane-bounded vesicles from a donor to an acceptor membrane. While there are many membrane remodelling complexes in eukaryotes, COPII, COPI, and clathrin-coated vesicles are the three principal classes of coat protein complexes that participate in vesicle trafficking in the endocytic and secretory pathways. These vesicle-coat proteins perform two key functions: deforming lipid bilayers into vesicles and encasing selective cargoes. The three trafficking complexes share some commonalities in their structural features but differ in their coat structures, mechanisms of cargo sorting, vesicle formation, and scission. While the structures of many of the proteins involved in vesicle formation have been determined in isolation by X-ray crystallography, elucidating the proteins' structures together with the membrane is better suited for cryogenic electron microscopy (cryo-EM). In recent years, advances in cryo-EM have led to solving the structures and mechanisms of several vesicle trafficking complexes and associated proteins.

摘要

真核细胞的膜性隔室之间的蛋白质运输是通过膜结合囊泡从供体膜到受体膜的不断分裂和融合来介导的。虽然真核生物中有许多膜重塑复合物,但 COPII、COPI 和网格蛋白包被的囊泡是参与内吞和分泌途径中囊泡运输的三种主要的包被蛋白复合物。这些囊泡包被蛋白执行两个关键功能:将脂质双层变形为囊泡并包裹选择性货物。这三个运输复合物在结构特征上具有一些共同性,但在包被结构、货物分拣机制、囊泡形成和分裂方面有所不同。虽然许多参与囊泡形成的蛋白质的结构已经通过 X 射线晶体学单独确定,但与膜一起阐明蛋白质的结构更适合低温电子显微镜(cryo-EM)。近年来,cryo-EM 的进步导致了几个囊泡运输复合物及其相关蛋白的结构和机制的解决。

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