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双调蛋白和表皮生长因子(EGF)促有丝分裂信号传导中对EGF受体COOH末端区域的不同需求。

A differential requirement for the COOH-terminal region of the epidermal growth factor (EGF) receptor in amphiregulin and EGF mitogenic signaling.

作者信息

Wong L, Deb T B, Thompson S A, Wells A, Johnson G R

机构信息

Division of Cytokine Biology, Center for Biologics Evaluation and Research, Food and Drug Administration, Bethesda, Maryland 20892, USA.

出版信息

J Biol Chem. 1999 Mar 26;274(13):8900-9. doi: 10.1074/jbc.274.13.8900.

DOI:10.1074/jbc.274.13.8900
PMID:10085134
Abstract

The epidermal growth factor receptor (EGFR) mediates the actions of a family of bioactive peptides that include epidermal growth factor (EGF) and amphiregulin (AR). Here we have studied AR and EGF mitogenic signaling in EGFR-devoid NR6 fibroblasts that ectopically express either wild type EGFR (WT) or a truncated EGFR that lacks the three major sites of autophosphorylation (c'1000). COOH-terminal truncation of the EGFR significantly impairs the ability of AR to (i) stimulate DNA synthesis, (ii) elicit Elk-1 transactivation, and (iii) generate sustained enzymatic activation of mitogen-activated protein kinase. EGFR truncation had no significant effect on AR binding to receptor but did result in defective GRB2 adaptor function. In contrast, EGFR truncation did not impair EGF mitogenic signaling, and in c'1000 cells EGF was able to stimulate the association of ErbB2 with GRB2 and SHC. Elk-1 transactivation was monitored when either ErbB2 or a truncated dominant-negative ErbB2 mutant (ErbB2-(1-813)) was overexpressed in cells. Overexpression of full-length ErbB2 resulted in a strong constitutive transactivation of Elk-1 in c'1000 but only slightly stimulated Elk-1 in WT or parental NR6 cells. Conversely, overexpression of ErbB2-(1-813) inhibited EGF-stimulated Elk-1 transactivation in c'1000 but not in WT cells. Thus, the cytoplasmic tail of the EGFR plays a critical role in AR mitogenic signaling but is dispensable for EGF, since EGF-activated truncated EGFRs can signal through ErbB2.

摘要

表皮生长因子受体(EGFR)介导包括表皮生长因子(EGF)和双调蛋白(AR)在内的一类生物活性肽的作用。在此,我们研究了在异位表达野生型EGFR(WT)或缺乏三个主要自磷酸化位点的截短型EGFR(c'1000)的无EGFR的NR6成纤维细胞中AR和EGF的促有丝分裂信号传导。EGFR的羧基末端截短显著损害了AR的以下能力:(i)刺激DNA合成,(ii)引发Elk-1反式激活,以及(iii)产生丝裂原活化蛋白激酶的持续酶促激活。EGFR截短对AR与受体的结合没有显著影响,但确实导致GRB2衔接蛋白功能缺陷。相比之下,EGFR截短并不损害EGF促有丝分裂信号传导,并且在c'1000细胞中EGF能够刺激ErbB2与GRB2和SHC的结合。当全长ErbB2或截短的显性负性ErbB2突变体(ErbB2-(1-813))在细胞中过表达时,监测Elk-1反式激活。全长ErbB2的过表达在c'1000中导致Elk-1的强烈组成型反式激活,但在WT或亲本NR6细胞中仅轻微刺激Elk-1。相反,ErbB2-(1-813)的过表达在c'1000中抑制EGF刺激的Elk-1反式激活,但在WT细胞中没有。因此,EGFR的细胞质尾巴在AR促有丝分裂信号传导中起关键作用,但对于EGF是可有可无的,因为EGF激活的截短型EGFR可以通过ErbB2发出信号。

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