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Generation of endogenous pH-sensitive EGF receptor and its application in high-throughput screening for proteins involved in clathrin-mediated endocytosis

机译:内源性pH敏感EGF受体的产生及其在网格蛋白介导的内吞作用相关蛋白的高通量筛选中的应用

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摘要

Previously we used gene-editing to label endogenous EGF receptor (EGFR) with GFP and demonstrate that picomolar concentrations of EGFR ligand drive signaling and endocytosis of EGFR in tumors in vivo (Pinilla-Macua et al., 2017). We now use gene-editing to insert a fluorogen activating protein (FAP) in the EGFR extracellular domain. Binding of the tandem dye pair MG-Bis-SA to FAP-EGFR provides a ratiometric pH-sensitive model with dual fluorescence excitation and a single far-red emission. The excitation ratio of fluorescence intensities was demonstrated to faithfully report the fraction of FAP-EGFR located in acidic endosomal/lysosomal compartments. Coupling native FAP-EGFR expression with the high method sensitivity has allowed development of a high-throughput assay to measure the rates of clathrin-mediated FAP-EGFR endocytosis stimulated with physiological EGF concentrations. The assay was utilized to screen a phosphatase siRNA library. These studies highlight the utility of endogenous pH-sensitive FAP-receptor chimeras in high-throughput analysis of endocytosis.
机译:以前,我们使用基因编辑功能以GFP标记内源性EGF受体(EGFR),并证明了皮摩尔浓度的EGFR配体在体内驱动肿瘤中EGFR的信号传导和内吞作用(Pinilla-Macua等人,2017)。现在,我们使用基因编辑在EGFR细胞外域中插入氟激活蛋白(FAP)。串联染料对MG-Bis-SA与FAP-EGFR的结合提供了一种具有双荧光激发和单远红外发射的比例pH敏感模型。已证明荧光强度的激发比忠实报告了位于酸性内体/溶酶体区室的FAP-EGFR分数。将天然的FAP-EGFR表达与高方法灵敏度相结合,已允许开发一种高通量检测方法,以测量生理EGF浓度刺激的网格蛋白介导的FAP-EGFR内吞率。该测定法用于筛选磷酸酶siRNA文库。这些研究突出了内源性pH敏感性FAP受体嵌合体在高通量内吞作用分析中的实用性。

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