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大鼠肝脏中胰岛素信号抑制剂Grb14的区室化及体内胰岛素诱导的易位

Compartmentalization and in vivo insulin-induced translocation of the insulin-signaling inhibitor Grb14 in rat liver.

作者信息

Desbuquois Bernard, Béréziat Véronique, Authier François, Girard Jean, Burnol Anne-Françoise

机构信息

Institut Cochin, Université Paris Descartes, CNRS UMR 8104, Paris, France.

出版信息

FEBS J. 2008 Sep;275(17):4363-77. doi: 10.1111/j.1742-4658.2008.06583.x. Epub 2008 Jul 24.

DOI:10.1111/j.1742-4658.2008.06583.x
PMID:18657188
Abstract

The molecular adaptor Grb14 binds in vitro to the activated insulin receptor (IR) and inhibits IR signaling. In this study, we have used rat liver subcellular fractionation to analyze in vivo insulin effects on Grb14 compartmentalization and IR phosphorylation and activity. In control rats, Grb14 was recovered mainly in microsomal and cytosolic fractions, but was also detectable at low levels in plasma membrane and Golgi/endosome fractions. Insulin injection led to a rapid and dose-dependent increase in Grb14 content, first in the plasma membrane fraction, and then in the Golgi/endosome fraction, which paralleled the increase in IR beta-subunit tyrosine phosphorylation. Upon sustained in vivo IR tyrosine phosphorylation induced by high-affinity insulin analogs, in vitro IR dephosphorylation by endogenous phosphatases, and in vivo phosphorylation of the IR induced by injection of bisperoxo(1,10 phenanthroline)oxovanadate, a phosphotyrosine phosphatase inhibitor, we observed a striking correlation between IR phosphorylation state and Grb14 content in both the plasma membrane and Golgi/endosome fractions. In addition, coimmunoprecipitation experiments provided evidence that Grb14 was associated with phosphorylated IR beta-subunit in these fractions. Altogether, these data support a model whereby insulin stimulates the recruitment of endogenous Grb14 to the activated IR at the plasma membrane, and induces internalization of the Grb14-IR complex in endosomes. Removal of Grb14 from fractions of insulin-treated rats by KCl treatment led to an increase of in vivo insulin-stimulated IR tyrosine kinase activity, indicating that endogenous Grb14 exerts a negative feedback control on IR catalytic activity. This study thus demonstrates that Grb14 is a physiological regulator of liver insulin signaling.

摘要

分子衔接蛋白Grb14在体外可与活化的胰岛素受体(IR)结合并抑制IR信号传导。在本研究中,我们利用大鼠肝脏亚细胞分级分离法来分析体内胰岛素对Grb14区室化以及IR磷酸化和活性的影响。在对照大鼠中,Grb14主要在微粒体和胞质组分中回收,但在质膜和高尔基体/内体组分中也可检测到低水平的Grb14。胰岛素注射导致Grb14含量迅速且呈剂量依赖性增加,首先在质膜组分中增加,然后在高尔基体/内体组分中增加,这与IRβ亚基酪氨酸磷酸化的增加平行。在高亲和力胰岛素类似物诱导的体内IR酪氨酸持续磷酸化、内源性磷酸酶对IR的体外去磷酸化以及注射磷酸酪氨酸磷酸酶抑制剂双过氧(1,10菲咯啉)氧钒酸盐诱导的IR体内磷酸化后,我们观察到质膜和高尔基体/内体组分中IR磷酸化状态与Grb14含量之间存在显著相关性。此外,免疫共沉淀实验提供了证据,表明在这些组分中Grb14与磷酸化的IRβ亚基相关联。总之,这些数据支持了一种模型,即胰岛素刺激内源性Grb14在质膜上募集到活化的IR,并诱导Grb14-IR复合物在内体中内化。通过KCl处理从胰岛素处理大鼠的组分中去除Grb14导致体内胰岛素刺激的IR酪氨酸激酶活性增加,表明内源性Grb14对IR催化活性发挥负反馈控制作用。因此,本研究证明Grb14是肝脏胰岛素信号传导的生理调节因子。

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