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葡萄糖转运蛋白GLUT4的内吞作用由GTP酶发动蛋白介导。

Endocytosis of the glucose transporter GLUT4 is mediated by the GTPase dynamin.

作者信息

Al-Hasani H, Hinck C S, Cushman S W

机构信息

Experimental Diabetes, Metabolism, and Nutrition Section, Diabetes Branch, NIDDK, National Institutes of Health, Bethesda, Maryland 20892, USA.

出版信息

J Biol Chem. 1998 Jul 10;273(28):17504-10. doi: 10.1074/jbc.273.28.17504.

DOI:10.1074/jbc.273.28.17504
PMID:9651341
Abstract

To study the role of the GTPase dynamin in GLUT4 intracellular recycling, we have overexpressed dynamin-1 wild type and a GTPase-negative mutant (K44A) in primary rat adipose cells. Transfection was accomplished by electroporation using an hemagglutinin (HA)-tagged GLUT4 as a reporter protein. In cells expressing HA-GLUT4 alone, insulin results in an approximately 7-fold increase in cell surface anti-HA antibody binding. Studies with wortmannin indicate that the kinetics of HA-GLUT4-trafficking parallel those of the native GLUT4 and in addition, that newly synthesized HA-GLUT4 goes to the plasma membrane before being sorted into the insulin-responsive compartments. Short term (4 h) coexpression of dynamin-K44A and HA-GLUT4 increases the amount of cell surface HA-GLUT4 in both the basal and insulin-stimulated states. Under conditions of maximal expression of dynamin-K44A (24 h), most or all of the intracellular HA-GLUT4 appears to be present on the cell surface in the basal state, and insulin has no further effect. Measurements of the kinetics of HA-GLUT4 endocytosis show that dynamin-K44A blocks internalization of the glucose transporters. In contrast, expression of dynamin wild type decreases the amount of cell surface HA-GLUT4 in both the basal and insulin-stimulated states. These data demonstrate that the endocytosis of GLUT4 is largely mediated by processes which require dynamin.

摘要

为研究GTP酶发动蛋白在葡萄糖转运蛋白4(GLUT4)细胞内再循环中的作用,我们在原代大鼠脂肪细胞中过表达了发动蛋白-1野生型和一种GTP酶阴性突变体(K44A)。使用带有血凝素(HA)标签的GLUT4作为报告蛋白,通过电穿孔完成转染。在仅表达HA-GLUT4的细胞中,胰岛素使细胞表面抗HA抗体结合增加约7倍。用渥曼青霉素进行的研究表明,HA-GLUT4转运的动力学与天然GLUT4的动力学相似,此外,新合成的HA-GLUT4在被分选到胰岛素反应性区室之前先到达质膜。发动蛋白-K44A与HA-GLUT4短期(4小时)共表达增加了基础状态和胰岛素刺激状态下细胞表面HA-GLUT4的量。在发动蛋白-K44A最大表达(24小时)的条件下,大多数或所有细胞内HA-GLUT4在基础状态下似乎都存在于细胞表面,胰岛素没有进一步作用。对HA-GLUT4内吞作用动力学的测量表明,发动蛋白-K44A阻断了葡萄糖转运体的内化。相反,发动蛋白野生型的表达在基础状态和胰岛素刺激状态下均降低了细胞表面HA-GLUT4的量。这些数据表明,GLUT4的内吞作用很大程度上由需要发动蛋白的过程介导。

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