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体外折叠人 G 蛋白偶联 Y2 受体到脂质环境的重构方案。

A reconstitution protocol for the in vitro folded human G protein-coupled Y2 receptor into lipid environment.

机构信息

Institute of Medical Physics and Biophysics, University of Leipzig, Härtelstr. 16-18, D-04107 Leipzig, Germany.

出版信息

Biophys Chem. 2010 Aug;150(1-3):29-36. doi: 10.1016/j.bpc.2010.02.019. Epub 2010 Apr 8.

Abstract

Although highly resolved crystal structures of G protein-coupled receptors have become available within the last decade, the need for studying these molecules in their natural membrane environment, where the molecules are rather dynamic, has been widely appreciated. Solid-state NMR spectroscopy is an excellent method to study structure and dynamics of membrane proteins in their native lipid environment. We developed a reconstitution protocol for the uniformly (15)N labeled Y(2) receptor into a bicelle-like lipid structure with high yields suitable for NMR studies. Milligram quantities of target protein were expressed in Escherichia coli using an optimized fermentation process in defined medium yielding in over 10mg/L medium of purified Y(2) receptor solubilized in SDS micelles. The structural integrity of the receptor molecules was strongly increased through refolding and subsequent reconstitution into phospholipid membranes. Specific ligand binding to the integrated receptor was determined using radioligand affinity assay. Further, by NMR measurement a dispersion of the (15)N signals comparable to native rhodopsin was shown. The efficiency of the reconstitution could also be inferred from the fact that reasonable (13)C NMR spectra at natural abundance could be acquired.

摘要

虽然在过去十年中已经获得了高分辨率的 G 蛋白偶联受体晶体结构,但人们广泛认识到需要在这些分子的自然膜环境中研究它们,因为这些分子相当动态。固态 NMR 光谱学是研究天然脂质环境中膜蛋白结构和动力学的极好方法。我们开发了一种将均匀(15)N 标记的 Y(2)受体重新组装到具有高产量的类似双分子层的脂质结构中的方案,适用于 NMR 研究。使用优化的发酵工艺在定义的培养基中在大肠杆菌中表达毫克级的目标蛋白,产量超过 10mg/L 培养基,其中含有溶解在 SDS 胶束中的纯化 Y(2)受体。通过复性和随后重新组装到磷脂膜中,大大增加了受体分子的结构完整性。通过放射性配体结合测定确定了整合受体的特异性配体结合。此外,通过 NMR 测量显示出与天然视紫红质相当的(15)N 信号的分散性。通过合理地获得天然丰度的(13)C NMR 谱也可以推断出重组成效。

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