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蛋白质组学揭示了表皮生长因子依赖性早期内体中与新型蛋白质的关联。

Proteomics reveals novel protein associations with early endosomes in an epidermal growth factor-dependent manner.

机构信息

From the Departments of Pharmacology and Toxicology and.

Medicine, University of Louisville, Louisville, Kentucky 40202.

出版信息

J Biol Chem. 2018 Apr 20;293(16):5895-5908. doi: 10.1074/jbc.RA117.000632. Epub 2018 Mar 9.

Abstract

The epidermal growth factor receptor (EGFR) is a receptor tyrosine kinase that is an integral component of proliferative signaling. EGFRs on the cell surface become activated upon EGF binding and have an increased rate of endocytosis. Once in the cytoplasm, the EGF·EGFR complex is trafficked to the lysosome for degradation, and signaling is terminated. During trafficking, the EGFR kinase domain remains active, and the internalized EGFR can continue signaling to downstream effectors. Although effector activity varies based on the EGFR's endocytic location, it is not clear how this occurs. In an effort to identify proteins that uniquely associate with the internalized, liganded EGFR in the early endosome, we developed an early endosome isolation strategy to analyze their protein composition. Post-nuclear supernatant from HeLa cells stimulated with and without EGF were separated on an isotonic 17% Percoll gradient. The gradient was fractionated, and early endosomal fractions were pooled and immunoisolated with an EEA1 mAb. The isolated endosomes were validated by immunoblot using antibodies against organelle-specific marker proteins and transmission EM. These early endosomes were also subjected to LC-MS/MS for proteomic analysis. Five proteins were detected in endosomes in a ligand-dependent manner: EGFR, RUFY1, STOML2, PTPN23, and CCDC51. Knockdown of RUFY1 or PTPN23 by RNAi indicated that both proteins play a role in EGFR trafficking. These experiments indicate that endocytic trafficking of activated EGFR changes the protein composition, membrane trafficking, and signaling potential of the early endosome.

摘要

表皮生长因子受体(EGFR)是一种受体酪氨酸激酶,是增殖信号的组成部分。细胞表面的 EGFRs 在 EGF 结合后被激活,内吞作用的速率增加。一旦进入细胞质,EGF·EGFR 复合物被运往溶酶体进行降解,信号被终止。在运输过程中,EGFR 激酶结构域保持活跃,内化的 EGFR 可以继续向下游效应物传递信号。尽管效应物的活性取决于 EGFR 的内吞位置,但目前尚不清楚这是如何发生的。为了鉴定与早期内体中内化的配体结合的 EGFR 独特相关的蛋白质,我们开发了一种早期内体分离策略来分析其蛋白质组成。用 EGF 刺激和未刺激的 HeLa 细胞的核后上清液在等渗 17%Percoll 梯度上分离。梯度被分馏,早期内体部分被汇集并使用 EEA1 mAb 免疫分离。通过针对细胞器特异性标记蛋白的免疫印迹和透射电镜验证分离的内体。这些早期内体也进行了 LC-MS/MS 蛋白质组学分析。有 5 种蛋白质以配体依赖的方式在内体中被检测到:EGFR、RUFY1、STOML2、PTPN23 和 CCDC51。通过 RNAi 敲低 RUFY1 或 PTPN23 表明这两种蛋白质都在 EGFR 运输中发挥作用。这些实验表明,激活的 EGFR 的内吞运输改变了早期内体的蛋白质组成、膜运输和信号转导潜力。

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