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Endocytic down-regulation of ErbB2 is stimulated by cleavage of its C-terminus

机译:内切性下调ErbB2的C端刺激。

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摘要

High ErbB2 levels are associated with cancer, and impaired endocytosis of ErbB2 could contribute to its overexpression. Therefore, knowledge about the mechanisms underlying endocytic down-regulation of ErbB2 is warranted. The C-terminus of ErbB2 can be cleaved after various stimuli, and after inhibition of HSP90 with geldanamycin this cleavage is accompanied by proteasome-dependent endocytosis of ErbB2. However, it is unknown whether C-terminal cleavage is linked to endocytosis. To study ErbB2 cleavage and endocytic trafficking, we fused yellow fluorescent protein (YFP) and cyan fluorescent protein (CFP) to the N- and C-terminus of ErbB2, respectively (YFP-ErbB2-CFP). After geldanamycin stimulation YFP-ErbB2-CFP became cleaved in nonapoptotic cells in a proteasome-dependent manner, and a markedly larger relative amount of cleaved YFP-ErbB2-CFP was observed in early endosomes than in the plasma membrane. Furthermore, cleavage took place at the plasma membrane, and cleaved ErbB2 was internalized and degraded far more efficiently than full-length ErbB2. Concordantly, a C-terminally truncated ErbB2 was also readily endocytosed and degraded in lysosomes compared with full-length ErbB2. Altogether, we suggest that geldanamycin leads to C-terminal cleavage of ErbB2, which releases the receptor from a retention mechanism and causes endocytosis and lysosomal degradation of ErbB2.
机译:高ErbB2水平与癌症有关,ErbB2的内吞能力受损可能会导致其过表达。因此,有必要了解有关ErbB2内吞性下调的机制。 ErbB2的C末端可以在各种刺激后被切割,并且在用格尔德霉素抑制HSP90后,这种切割伴随着蛋白酶体依赖性的ErbB2内吞作用。但是,尚不知道C末端的切割是否与内吞作用有关。为了研究ErbB2的切割和胞吞运输,我们将黄色荧光蛋白(YFP)和青色荧光蛋白(CFP)分别融合到ErbB2的N和C端(YFP-ErbB2-CFP)。格尔德霉素刺激后,YFP-ErbB2-CFP在非凋亡细胞中以蛋白酶体依赖性方式被裂解,并且在早期内体中观察到的裂解的YFP-ErbB2-CFP相对量明显大于质膜。此外,裂解在质膜处发生,并且裂解的ErbB2比全长ErbB2更有效地内化和降解。相应地,与全长ErbB2相比,C端截短的ErbB2在溶酶体中也很容易被内吞并降解。总而言之,我们建议格尔德霉素导致ErbB2的C末端裂解,从而从保留机制中释放受体,并引起ErbB2的内吞作用和溶酶体降解。

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