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通过整合到纳米级脂质双层中来直接溶解异源表达的膜蛋白。

Direct solubilization of heterologously expressed membrane proteins by incorporation into nanoscale lipid bilayers.

作者信息

Civjan Natanya R, Bayburt Timothy H, Schuler Mary A, Sligar Stephen G

机构信息

Department of Biochemistry, University of Illinois, 505 S. Goodwin Avenue, Urbana, IL 61801, USA.

出版信息

Biotechniques. 2003 Sep;35(3):556-60, 562-3. doi: 10.2144/03353rr02.

Abstract

One of the biggest challenges in the field of proteomics is obtaining functional membrane proteins solubilized and dispersed into a physiologically relevant environment that maintains the spectrum of in vivo activities. Here we describe a system composed of nanoscale self-assembled particles, termed Nanodiscs, which contain a single phospholipid bilayer stabilized by an encircling membrane scaffold protein (MSP). Using microsomal membranes of baculovirus-infected Spodoptera frugiperda (Sf9) insect cells overexpressing an N-terminally anchored cytochrome P450 monoxygenase (P450), we demonstrate that target membrane proteins can be directly solubilized and incorporated into distinct populations of Nanodiscs, which can be separated by size chromatography. We show that formation of these Nanodiscs from insect cell membranes allows for the compartmentalization into soluble nanostructures that provide a natural membrane bilayer that avoids the aggregation of membrane proteins often encountered in other reconstitution procedures. Lipid composition analysis and substrate binding analysis of size-fractionated Nanodiscs arrayed in microtiter plates further demonstrates that the Nanodisc system effectively disperses the overexpressed membrane protein into monodispersed bilayers containing biochemically defined lipid components and the target protein in its native from suitable for sensitive high-throughput substrate binding analysis.

摘要

蛋白质组学领域最大的挑战之一是获得溶解并分散在生理相关环境中的功能性膜蛋白,该环境能维持体内活性谱。在此,我们描述了一种由纳米级自组装颗粒组成的系统,称为纳米圆盘(Nanodiscs),它包含一个由环绕的膜支架蛋白(MSP)稳定的单一磷脂双层。使用过表达N端锚定细胞色素P450单加氧酶(P450)的杆状病毒感染的草地贪夜蛾(Sf9)昆虫细胞的微粒体膜,我们证明目标膜蛋白可以直接溶解并整合到不同群体的纳米圆盘中,这些纳米圆盘可以通过尺寸色谱法分离。我们表明,从昆虫细胞膜形成这些纳米圆盘允许分隔成可溶性纳米结构,提供天然膜双层,避免了在其他重组程序中经常遇到的膜蛋白聚集。对排列在微量滴定板中的尺寸分级纳米圆盘进行脂质组成分析和底物结合分析进一步证明,纳米圆盘系统有效地将过表达的膜蛋白分散到含有生化定义脂质成分的单分散双层中,并且目标蛋白以其天然形式存在,适合进行灵敏的高通量底物结合分析。

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