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Fluorescence-based methods to image palmitoylated proteins.

机译:基于荧光的方法对棕榈酰化蛋白进行成像。

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摘要

A well known function of palmitoylation is to promote protein binding to cell membranes. Until recently, it was unclear what additional roles, if any, palmitoylation has in controlling protein localization in cells. Recent studies of palmitoylated forms of the small GTPase Ras have now revealed that palmitoylation plays multiple roles in the regulation of protein trafficking, including targeting proteins into the secretory pathway and recycling proteins between the plasma membrane and Golgi complex. We here describe how quantitative fluorescence microscopy and photobleaching approaches can be used to study the intracellular targeting and trafficking of GFP-tagged palmitoylated proteins in living cells. We discuss (1) general considerations for fluorescence recovery after photobleaching (FRAP) measurements of GFP-tagged proteins; (2) FRAP-based assays to test the strength of binding of palmitoylated proteins to cell membranes; (3) methods to establish the kinetics and mechanisms of recycling of palmitoylated proteins between the Golgi complex and the plasma membrane; (4) the use of the palmitoylation inhibitor 2-bromo-palmitate as a tool to study the dynamic regulation of protein targeting and trafficking by palmitate turnover.
机译:棕榈酰化的众所周知的功能是促进蛋白质与细胞膜的结合。直到最近,还不清楚棕榈酰化在控制细胞中蛋白质定位方面还有哪些其他作用(如果有的话)。近期对小GTP酶Ras的棕榈酰化形式的研究表明,棕榈酰化在调节蛋白运输中起多种作用,包括将蛋白靶向到分泌途径中以及在质膜和高尔基复合体之间再循环蛋白。我们在这里描述如何定量荧光显微镜和光漂白方法可用于研究活细胞中GFP标记的棕榈酰化蛋白的细胞内靶向和运输。我们讨论(1)对带有GFP标签的蛋白进行光漂白(FRAP)测量后荧光恢复的一般考虑; (2)基于FRAP的检测方法,以测试棕榈酰化蛋白与细胞膜的结合强度; (3)建立高尔基复合体和质膜之间棕榈酰化蛋白循环动力学和机制的方法; (4)使用棕榈酰化抑制剂2-溴-棕榈酸酯作为研究棕榈酸酯周转对蛋白质靶向和运输的动态调节的工具。

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