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转染细胞衍生的巨大囊泡中定量的曲率和相诱导的蛋白质分选。

Curvature- and Phase-Induced Protein Sorting Quantified in Transfected Cell-Derived Giant Vesicles.

机构信息

Niels Bohr Institute , University of Copenhagen , DK-2100 Copenhagen , Denmark.

Department of Biochemistry and Biophysics , Stockholm University , 10691 Stockholm , Sweden.

出版信息

ACS Nano. 2019 Jun 25;13(6):6689-6701. doi: 10.1021/acsnano.9b01052. Epub 2019 Jun 14.

DOI:10.1021/acsnano.9b01052
PMID:31199124
Abstract

Eukaryotic cells possess a dynamic network of membranes that vary in lipid composition. To perform numerous biological functions, cells modulate their shape and the lateral organization of proteins associated with membranes. The modulation is generally facilitated by physical cues that recruit proteins to specific regions of the membrane. Analyzing these cues is difficult due to the complexity of the membrane conformations that exist in cells. Here, we examine how different types of membrane proteins respond to changes in curvature and to lipid phases found in the plasma membrane. By using giant plasma membrane vesicles derived from transfected cells, the proteins were positioned in the correct orientation and the analysis was performed in plasma membranes with a biological composition. Nanoscale membrane curvatures were generated by extracting nanotubes from these vesicles with an optical trap. The viral membrane protein neuraminidase was not sensitive to curvature, but it did exhibit strong partitioning (coefficient of K = 0.16) disordered membrane regions. In contrast, the membrane repair protein annexin 5 showed a preference for nanotubes with a density up to 10-15 times higher than that on the more flat vesicle membrane. The investigation of nanoscale effects in isolated plasma membranes provides a quantitative platform for studying peripheral and integral membrane proteins in their natural environment.

摘要

真核细胞拥有动态的膜网络,其脂质组成各不相同。为了执行众多生物学功能,细胞会调节其形状和与膜相关的蛋白质的侧向组织。这种调节通常是通过物理线索来实现的,这些线索将蛋白质募集到膜的特定区域。由于细胞中存在的膜构象的复杂性,分析这些线索具有一定的难度。在这里,我们研究了不同类型的膜蛋白如何响应曲率变化以及质膜中存在的脂质相的变化。通过使用源自转染细胞的巨大质膜囊泡,将蛋白质定位在正确的方向,并在具有生物学组成的质膜中进行分析。通过用光阱从这些囊泡中提取纳米管来产生纳米级的膜曲率。病毒膜蛋白神经氨酸酶对曲率不敏感,但它确实表现出强烈的分区(系数 K = 0.16)无序膜区域。相比之下,膜修复蛋白 annexin 5 对纳米管表现出偏好,其密度比更平坦的囊泡膜高 10-15 倍。在分离的质膜中研究纳米级效应为在其自然环境中研究外周和整合膜蛋白提供了一个定量平台。

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