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In Situ Quantification of Protein Binding to the Plasma Membrane

机译:蛋白质与血浆膜结合的原位定量

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摘要

This study presents a fluorescence-based assay that allows for direct measurement of protein binding to the plasma membrane inside living cells. An axial scan through the cell generates a fluorescence intensity profile that is analyzed to determine the membrane-bound and cytoplasmic concentrations of a peripheral membrane protein labeled by the enhanced green fluorescent protein (EGFP). The membrane binding curve is constructed by mapping those concentrations for a population of cells with a wide range of protein expression levels, and a fit of the binding curve determines the number of binding sites and the dissociation coefficient. We experimentally verified the technique, using myosin-1C-EGFP as a model system and fit its binding curve. Furthermore, we studied the protein-lipid interactions of the membrane binding domains from lactadherin and phospholipase C-δ1 to evaluate the feasibility of using competition binding experiments to identify specific lipid-protein interactions in living cells. Finally, we applied the technique to determine the lipid specificity, the number of binding sites, and the dissociation coefficient of membrane binding for the Gag matrix domain of human T-lymphotropic virus type 1, which provides insight into early assembly steps of the retrovirus.
机译:这项研究提出了一种基于荧光的检测方法,可以直接测量与活细胞内部质膜结合的蛋白质。通过细胞的轴向扫描产生荧光强度分布图,对其进行分析以确定由增强的绿色荧光蛋白(EGFP)标记的外周膜蛋白的膜结合浓度和细胞质浓度。膜结合曲线是通过绘制那些浓度范围广泛的具有蛋白质表达水平的细胞群体的浓度而绘制的,结合曲线的拟合度决定了结合位点的数量和解离系数。我们使用肌球蛋白-1C-EGFP作为模型系统,通过实验验证了该技术,并拟合了其结合曲线。此外,我们研究了来自乳黏附素和磷脂酶C-δ1的膜结合域的蛋白质-脂质相互作用,以评估使用竞争结合实验鉴定活细胞中特定脂质-蛋白质相互作用的可行性。最后,我们应用了该技术来确定人T淋巴病毒1型的Gag基质域的脂质特异性,结合位点的数量和膜结合的解离系数,从而为逆转录病毒的早期组装步骤提供了见识。

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