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Sonic hedgehog 独立于经典 hedgehog 信号激活 Erk。

Activation of Erk by sonic hedgehog independent of canonical hedgehog signalling.

机构信息

Department of Laboratory Medicine and Pathobiology, Faculty of Medicine, University of Toronto, Toronto, Ontario, Canada.

出版信息

Int J Biochem Cell Biol. 2010 Sep;42(9):1462-71. doi: 10.1016/j.biocel.2010.04.016. Epub 2010 May 6.

Abstract

Hedgehog (Hh) signalling is mediated through the Patched-1 (Ptch1) receptor. Hh-binding to Ptch1 blocks the inhibitory effects of Ptch1 on the activity of the transmembrane protein, Smoothened (Smo), resulting induction of target genes by the Gli-family of transcription factors. We demonstrate here that Hh-binding to Ptch1 stimulates activation of Erk1/2. This activation is insensitive to the small molecule Smo antagonists and occurs in a cell line that does not express Smo. Specifically, the C-terminus of Ptch1 harbours motifs encoding Class I and II SH3-binding sites. SH3-domain binding activity was verified using GST-c-src(SH3), -Grb2(SH3) and -p85beta(SH3) fusion-proteins. Ectopically expressed Grb2 or p85beta could also be co-immunoprecipitated with the Ptch1 C-terminus. Addition of Shh to serum-starved human mammary epithelial cells and Shh Light II fibroblasts stimulated phosphorylation of Erk1/2. Erk1/2 activation was observed in cells where Smo activity had been inhibited using cyclopamine and in the breast epithelial cell line, MCF10A, that does not express Smo. These data reveal novel binding activities for the C-terminal region of Ptch1 and define a signalling pathway stimulated by the Hh-ligands operating independently of pathways requiring Smo.

摘要

Hedgehog (Hh) 信号通过 Patched-1 (Ptch1) 受体进行介导。Hh 与 Ptch1 的结合会阻止 Ptch1 对跨膜蛋白 Smoothened (Smo) 的抑制作用,从而诱导 Gli 转录因子家族的靶基因表达。我们在此证明 Hh 与 Ptch1 的结合会刺激 Erk1/2 的激活。这种激活对小分子 Smo 拮抗剂不敏感,并且发生在不表达 Smo 的细胞系中。具体而言,Ptch1 的 C 端含有编码 I 类和 II 类 SH3 结合基序的模体。使用 GST-c-src(SH3)、-Grb2(SH3) 和 -p85beta(SH3) 融合蛋白验证了 SH3 结构域结合活性。过表达的 Grb2 或 p85beta 也可以与 Ptch1 的 C 端共免疫沉淀。用 Shh 处理血清饥饿的人乳腺上皮细胞和 Shh Light II 成纤维细胞可刺激 Erk1/2 的磷酸化。在使用环巴胺抑制 Smo 活性的细胞中和在不表达 Smo 的乳腺上皮细胞系 MCF10A 中观察到 Erk1/2 的激活。这些数据揭示了 Ptch1 C 端的新结合活性,并定义了一条由 Hh 配体刺激的信号通路,该通路独立于需要 Smo 的途径。

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