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Genetically Encoded Spy Peptide Fusion System to Detect Plasma Membrane-Localized Proteins In Vivo

机译:基因编码的间谍肽融合系统,以检测体内血浆膜定位的蛋白质。

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摘要

Membrane proteins are the main gatekeepers of cellular state, especially in neurons, serving either to maintain homeostasis or instruct response to synaptic input or other external signals. Visualization of membrane protein localization and trafficking in live cells facilitates understanding the molecular basis of cellular dynamics. We describe here a method for specifically labeling the plasma membrane-localized fraction of heterologous membrane protein expression using channelrhodopsins as a case study. We show that the genetically encoded, covalent binding SpyTag and SpyCatcher pair from the Streptococcus pyogenes fibronectin-binding protein FbaB can selectively label membrane-localized proteins in living cells in culture and in vivo in Caenorhabditis elegans. The SpyTag/SpyCatcher covalent labeling method is highly specific, modular, and stable in living cells. We have used the binding pair to develop a channelrhodopsin membrane localization assay that is amenable to high-throughput screening for opsin discovery and engineering.
机译:膜蛋白是细胞状态(尤其是在神经元中)的主要守门员,其作用是维持体内稳态或指示对突触输入或其他外部信号的反应。膜蛋白在活细胞中的定位和运输的可视化有助于理解细胞动力学的分子基础。我们在这里描述了一种使用通道视紫红质作为案例研究特异性标记异源膜蛋白表达的质膜定位部分的方法。我们显示,从化脓性链球菌纤连蛋白结合蛋白FbaB的遗传编码,共价结合SpyTag和SpyCatcher对可以选择性地标记在秀丽隐杆线虫中培养和活体内的活细胞中的膜定位蛋白。 SpyTag / SpyCatcher共价标记方法在活细胞中高度特异性,模块化且稳定。我们已经使用结合对来开发通道视紫红质膜定位测定法,该测定法适合于高通量筛选视蛋白的发现和工程设计。

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