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磷脂双层纳米盘膜支架蛋白的构象转变。

Conformational transitions in the membrane scaffold protein of phospholipid bilayer nanodiscs.

机构信息

Department of Chemistry and Chemical Biology, Northeastern University, Boston, MA 02115, USA.

出版信息

Mol Cell Proteomics. 2011 Sep;10(9):M111.010876. doi: 10.1074/mcp.M111.010876. Epub 2011 Jun 29.

Abstract

Phospholipid bilayer nanodiscs are model membrane systems that provide an environment where membrane proteins are highly stable and monodisperse without the use of detergents or liposomes. Nanodiscs consist of a discoidal phospholipid bilayer encircled by two copies of an amphipathic alpha helical membrane scaffold protein, which is modeled from apolipoprotein A-1. Hydrogen exchange mass spectrometry was used to probe the structure and dynamics of the scaffold protein in the presence and absence of lipid. On nanodisc self-assembly, the entire scaffold protein gained significant protection from exchange, consistent with a large, protein-wide, structural rearrangement. This protection was short-lived and the scaffold protein was highly deuterated within 2 h. Several regions of the scaffold protein, in both the lipid-free and lipid-associated states, displayed EX1 unfolding kinetics. The rapid deuteration of the scaffold protein and the presence of correlated unfolding events both indicate that nanodiscs are dynamic rather than rigid bodies in solution. This work provides a catalog of the expected scaffold protein peptic peptides in a nanodisc-hydrogen exchange mass spectrometry experiment and their deuterium uptake signatures, data that can be used as a benchmark to verify correct assembly and nanodisc structure. Such reference data will be useful control data for all hydrogen exchange mass spectrometry experiments involving nanodiscs in which transmembrane or lipid-associated proteins are the primary molecule(s) of interest.

摘要

磷脂双层纳米盘是一种模型膜系统,它提供了一个环境,其中膜蛋白高度稳定且单分散,而无需使用去污剂或脂质体。纳米盘由一个双分子层的盘状磷脂双层组成,周围环绕着两个两亲性α螺旋膜支架蛋白拷贝,该蛋白是从载脂蛋白 A-1 模拟而来的。氢交换质谱法被用来探测支架蛋白在存在和不存在脂质的情况下的结构和动力学。在纳米盘自组装过程中,整个支架蛋白获得了显著的保护,免受交换的影响,这与一个大的、蛋白范围的结构重排一致。这种保护是短暂的,在 2 小时内,支架蛋白高度氘化。在无脂质和与脂质结合的状态下,支架蛋白的几个区域都显示出 EX1 展开动力学。支架蛋白的快速氘化和相关展开事件的存在都表明,纳米盘在溶液中是动态的,而不是刚性的。这项工作提供了在纳米盘-氢交换质谱实验中预期的支架蛋白肽的目录,以及它们的氘摄取特征,这些数据可作为验证正确组装和纳米盘结构的基准。对于所有涉及跨膜或与脂质结合的蛋白质是主要研究对象的纳米盘氢交换质谱实验,这种参考数据将是有用的控制数据。

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