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网格蛋白重链和α-衔接蛋白特异性小干扰RNA对HeLa细胞内吞辅助蛋白和受体转运的影响

Effect of clathrin heavy chain- and alpha-adaptin-specific small inhibitory RNAs on endocytic accessory proteins and receptor trafficking in HeLa cells.

作者信息

Hinrichsen Lars, Harborth Jens, Andrees Lars, Weber Klaus, Ungewickell Ernst J

机构信息

Department of Cell Biology in the Center of Anatomy, Hannover Medical School, D-30623 Hannover, Germany.

出版信息

J Biol Chem. 2003 Nov 14;278(46):45160-70. doi: 10.1074/jbc.M307290200. Epub 2003 Sep 6.

DOI:10.1074/jbc.M307290200
PMID:12960147
Abstract

To assess the contribution of individual endocytic proteins to the assembly of clathrin coated pits, we depleted the clathrin heavy chain and the alpha-adaptin subunit of AP-2 in HeLa-cells using RNA interference. 48 h after transfection with clathrin heavy chain-specific short interfering RNA both, the heavy and light chains were depleted by more than 80%. Residual clathrin was mainly membrane-associated, and an increase in shallow pits was noted. The membrane-association of adaptors, clathrin assembly lymphoid myeloid leukemia protein (CALM), epsin, dynamin, and Eps15 was only moderately affected by the knockdown and all proteins still displayed a punctate staining distribution. Clathrin depletion inhibited the uptake of transferrin but not that of the epidermal growth factor. However, efficient sorting of the epidermal growth factor into hepatocyte growth factor-regulated tyrosine kinase substrate-positive endosomes was impaired. Depletion of alpha-adaptin abolished almost completely the plasma membrane association of clathrin. Binding of Eps15 to membranes was strongly and that of CALM moderately reduced. Whereas the uptake of transferrin was efficiently blocked in alpha-adaptin knockdown cells, the internalization and sorting of the epidermal growth factor was not significantly impaired. Since neither clathrin nor AP-2 is essential for the internalization of EGF, we conclude that it is taken up by an alternative mechanism.

摘要

为了评估单个内吞蛋白对网格蛋白包被小窝组装的贡献,我们利用RNA干扰技术在HeLa细胞中敲低了网格蛋白重链和AP-2的α-衔接蛋白亚基。用网格蛋白重链特异性短干扰RNA转染48小时后,重链和轻链的表达均降低了80%以上。残留的网格蛋白主要与膜相关,并且观察到浅小窝数量增加。衔接蛋白、网格蛋白组装淋巴样髓样白血病蛋白(CALM)、epsin、发动蛋白和Eps15的膜结合仅受到敲低的中度影响,所有蛋白仍呈现点状染色分布。网格蛋白的缺失抑制了转铁蛋白的摄取,但不影响表皮生长因子的摄取。然而,表皮生长因子向肝细胞生长因子调节的酪氨酸激酶底物阳性内体的有效分选受到损害。α-衔接蛋白的缺失几乎完全消除了网格蛋白与质膜的结合。Eps15与膜的结合强烈减少,CALM与膜的结合中度减少。虽然在α-衔接蛋白敲低的细胞中转铁蛋白的摄取被有效阻断,但表皮生长因子的内化和分选没有受到明显损害。由于网格蛋白和AP-2对于表皮生长因子的内化都不是必需的,我们得出结论,它是通过一种替代机制被摄取的。

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