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通过大肠杆菌大机械敏感离子通道(MscL)的二维结晶揭示的六聚体跨膜孔。

A hexameric transmembrane pore revealed by two-dimensional crystallization of the large mechanosensitive ion channel (MscL) of Escherichia coli.

作者信息

Saint N, Lacapère J J, Gu L Q, Ghazi A, Martinac B, Rigaud J L

机构信息

Department of Pharmacology, University of Western Australia, Nedlands, WA 6907, Australia.

出版信息

J Biol Chem. 1998 Jun 12;273(24):14667-70. doi: 10.1074/jbc.273.24.14667.

Abstract

We have established a reconstitution method of the detergent-solubilized recombinant large mechanosensitive ion channel of Escherichia coli (MscL) that yielded two-dimensional crystals. For that purpose, we have developed a new protocol using Triton X-100 to solubilize and purify the MscL protein. This protocol not only allowed an increase in the protein yield but also made it possible to obtain a homogeneous delipidated and reproducible preparation of the purified protein. When examined by the patch-clamp method MscL channels were found to be fully functional, exhibiting characteristic conductance and activation by pressure. For electron crystallography the homogeneous Triton X-100-purified recombinant MscL was further reconstituted at low lipid-to-protein ratios using Bio-Beads SM2 to remove the detergent. Two-dimensional crystals, exhibiting a p6 plane group symmetry, have been produced and examined by negative stain electron microscopy. Image processing of selected micrographs yielded a projection map at 15-A resolution that provided the first explicit structural information about the molecular boundary and homohexameric organization of the MscL channels in the membrane bilayer.

摘要

我们建立了一种用于去污剂增溶的大肠杆菌大机械敏感离子通道(MscL)的重组方法,该方法可产生二维晶体。为此,我们开发了一种使用 Triton X-100 增溶和纯化 MscL 蛋白的新方案。该方案不仅提高了蛋白产量,还使得获得纯化蛋白的均一脱脂且可重复的制剂成为可能。通过膜片钳方法检测发现,MscL 通道功能完全正常,表现出特征性电导并可被压力激活。对于电子晶体学,使用 Bio-Beads SM2 在低脂质与蛋白比例下进一步重组均一的经 Triton X-100 纯化的重组 MscL,以去除去污剂。已制备出具有 p6 平面群对称性的二维晶体,并通过负染电子显微镜进行了检测。对选定显微照片的图像处理产生了分辨率为 15 埃的投影图,该图提供了关于膜双层中 MscL 通道分子边界和同六聚体组织的首个明确结构信息。

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