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无标记测量脂质膜中分子的扩散系数。

Label-free measurements of the diffusivity of molecules in lipid membranes.

机构信息

Department of Applied Physics, Chalmers University of Technology, 41296 Gothenburg (Sweden).

出版信息

Chemphyschem. 2014 Feb 24;15(3):486-91. doi: 10.1002/cphc.201301136. Epub 2014 Jan 8.

DOI:10.1002/cphc.201301136
PMID:24402971
Abstract

An important and characteristic property of a cell membrane is the lateral mobility of protein molecules in the lipid bilayer. This has conventionally been measured by labeling the molecules with fluorescent markers and monitoring their mobility by different fluorescence-based techniques. However, adding the label to the studied molecule may affect the system, so it is an assumption in almost all experiments that the measured mobility of the biomolecule with its label is the same as that of the unlabeled molecule. However, this assumption is rarely tested due to a lack of suitable methods. In this work, a new technique to perform label-free diffusivity measurements is developed and used to measure the effect of the label for two common protein-lipid systems: 1) streptavidin (SA) coupled to a supported lipid bilayer (SLB) through biotinylated lipids and 2) the extracellular part of the T-cell adhesion protein CD2, coupled to an SLB through histidine tags to nickel-chelating lipids. A measurable (≈12%) decrease in diffusivity is found for both labeled proteins, even though the molecular mass of the label is almost 100 times smaller than those of the proteins (≈50 kDa). The results illustrate the importance of being able to study different biophysical properties of cell membranes and their mimics without relying on fluorescent labels, especially if fluorescent labeling is difficult or is expected to affect the nature of the intermolecular interactions being studied.

摘要

细胞膜的一个重要和特征性质是蛋白质分子在脂质双层中的横向流动性。这通常通过用荧光标记物标记分子并通过不同的荧光技术监测其流动性来测量。然而,向被研究的分子添加标记物可能会影响系统,因此在几乎所有实验中都有一个假设,即带有标记的生物分子的测量流动性与其未标记的分子相同。然而,由于缺乏合适的方法,这个假设很少被检验。在这项工作中,开发了一种新的无标记扩散测量技术,并用于测量两种常见的蛋白质-脂质系统的标记物的影响:1)通过生物素化脂质偶联到支撑脂质双层(SLB)上的链霉亲和素(SA),2)通过组氨酸标签偶联到镍螯合脂质上的 T 细胞粘附蛋白 CD2 的细胞外部分。即使标记物的分子量几乎比蛋白质小 100 倍(约 50 kDa),两种标记蛋白的扩散性都有可测量的(≈12%)下降。这些结果说明了能够在不依赖荧光标记的情况下研究细胞膜及其模拟物的不同生物物理性质的重要性,特别是如果荧光标记困难或预计会影响正在研究的分子间相互作用的性质。

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