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插入到支撑脂质双分子层顶部的单拓扑膜蛋白的电泳迁移率。

Electrophoretic mobility of a monotopic membrane protein inserted into the top of supported lipid bilayers.

作者信息

Harb Frédéric, Giudici-Orticoni Marie-Thérèse, Guiral Marianne, Tinland Bernard

机构信息

Doctoral school for Science and Technology, platform for research in Nanosciences and Nanotechnology, Lebanese University, Campus Pierre Gemayel, BP 90239, Fanar-Metn, Lebanon.

Aix-Marseille Univ, CINaM-CNRS, UMR7325, 13288, Marseille, France.

出版信息

Eur Phys J E Soft Matter. 2016 Dec;39(12):127. doi: 10.1140/epje/i2016-16127-1. Epub 2016 Dec 21.

Abstract

We have studied the translational migration of a monotopic membrane protein, the bacterial sulfide quinone reductase (SQR) in supported n-bilayers ([Formula: see text]) under the influence of an electric field parallel to the membrane plane. The direction of the migration changes when the charge of the protein changes its sign. Measuring mobilities at different pH enables us to gain experimental physico-chemical data on SQR as its isoelectric point and its estimated oligomeric state (at least trimeric) when inserted in a lipid membrane. Consequently, in addition to the migration study of membrane proteins in a lipid environment, this experimental system, previously used with a transmembrane protein, is thus suitable to define membrane protein properties in conditions approaching the native ones (in the absence of detergent).

摘要

我们研究了单一位点膜蛋白——细菌硫化物醌还原酶(SQR)在平行于膜平面的电场影响下,在支撑的正双层膜([公式:见正文])中的平移迁移。当蛋白质的电荷改变其符号时,迁移方向会发生变化。在不同pH值下测量迁移率,使我们能够获得关于SQR的实验物理化学数据,如它的等电点以及插入脂质膜时其估计的寡聚状态(至少三聚体)。因此,除了研究膜蛋白在脂质环境中的迁移外,这个先前用于跨膜蛋白的实验系统,也适用于在接近天然条件(无去污剂)下定义膜蛋白的特性。

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