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在疏水基底上的转移和在平面脂双层中重组的膜蛋白的原子力显微镜成像。

Transfer on hydrophobic substrates and AFM imaging of membrane proteins reconstituted in planar lipid bilayers.

机构信息

Centre de Biochimie Structurale, CNRS UMR 5048, INSERM U554, UM1, UM2, Montpellier, France.

出版信息

J Mol Recognit. 2011 May-Jun;24(3):461-6. doi: 10.1002/jmr.1070.

Abstract

The lipid-layer technique allows reconstituting transmembrane proteins at a high density in microns size planar membranes and suspended to a lipid monolayer at the air/water interface. In this paper, we transferred these membranes onto two hydrophobic substrates for further structural analysis of reconstituted proteins by Atomic Force Microscopy (AFM). We used a mica sheet covered by a lipid monolayer or a sheet of highly oriented pyrolytic graphite (HOPG) to trap the lipid monolayer at the interface and the suspended membranes. In both cases, we succeeded in the transfer of large membrane patches containing densely packed or 2D-crystallized proteins. As a proof of concept, we transferred and imaged the soluble Shiga toxin bound to its lipid ligand and the ATP-binding cassette (ABC) transporter BmrA reconstituted into a planar bilayer. AFM imaging with a lateral resolution in the nanometer range was achieved. Potential applications of this technique in structural biology and nanobiotechnology are discussed.

摘要

脂质层技术允许在微米大小的平面膜中将跨膜蛋白以高密度重新构成,并悬浮在空气/水界面的单层脂质中。在本文中,我们将这些膜转移到两个疏水性基质上,以便通过原子力显微镜(AFM)对重新构成的蛋白质进行进一步的结构分析。我们使用覆盖有单层脂质的云母片或高度取向的热解石墨(HOPG)片来捕获界面处的单层脂质和悬浮的膜。在这两种情况下,我们都成功地转移了包含高密度或二维结晶蛋白质的大膜片。作为概念验证,我们转移并成像了与脂质配体结合的可溶性志贺毒素和重新构成的平面双层的 ATP 结合盒(ABC)转运蛋白 BmrA。实现了纳米级别的横向分辨率的 AFM 成像。讨论了该技术在结构生物学和纳米生物技术中的潜在应用。

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