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Smad7与激活素I型受体相互作用的磷酸化调节

Phosphorylation regulation of the interaction between Smad7 and activin type I receptor.

作者信息

Liu Xubao, Nagarajan Raman P, Vale Wylie, Chen Yan

机构信息

Department of Medical and Molecular Genetics and the Walther Oncology Center, Indiana University School of Medicine, and the Walther Cancer Institute, 975 West Walnut Street, IB130, Indianapolis, IN 46202, USA.

出版信息

FEBS Lett. 2002 May 22;519(1-3):93-8. doi: 10.1016/s0014-5793(02)02718-7.

DOI:10.1016/s0014-5793(02)02718-7
PMID:12023024
Abstract

Signal transduction of activin, one of the members in the transforming growth factor-beta superfamily, is initiated by ligand binding with two distinct membrane receptors (type II and type I) followed by activation of Smad2 or Smad3. We report here that activin-induced signaling is negatively regulated by another Smad molecule, Smad7. When expressed in Chinese hamster ovary cells, Smad7 inhibited the transcriptional response induced by either activin treatment or a constitutively active activin type I receptor (ALK-4). In addition, Smad7 also inhibited mouse FAST-2-mediated transactivation of the Xenopus Mix.2 promoter stimulated by the constitutively active ALK-4. Smad7 was able to directly associate with ALK-4 and this association was dependent on the phosphorylation of the type I receptor in its GS domain by activin type II receptors. Expression of kinase defective activin type II receptors decreased the association of Smad7 with ALK-4. Correspondingly, Smad7 bound poorly to a mutant ALK-4 bearing serine to alanine substitutions in four putative phosphorylation sites in its GS domain. These studies not only illustrated the counter regulatory function of Smad7 on activin signaling, but also indicated the involvement of phosphorylation at activin type I receptor in the inhibitory action of Smad7.

摘要

激活素是转化生长因子-β超家族的成员之一,其信号转导是由配体与两种不同的膜受体(II型和I型)结合启动,随后激活Smad2或Smad3。我们在此报告,激活素诱导的信号传导受到另一种Smad分子Smad7的负调控。当在中国仓鼠卵巢细胞中表达时,Smad7抑制了激活素处理或组成型活性激活素I型受体(ALK-4)诱导的转录反应。此外,Smad7还抑制了组成型活性ALK-4刺激的小鼠FAST-2介导的非洲爪蟾Mix.2启动子的反式激活。Smad7能够直接与ALK-4结合,这种结合依赖于激活素II型受体对I型受体GS结构域的磷酸化。激酶缺陷型激活素II型受体的表达减少了Smad7与ALK-4的结合。相应地,Smad7与在其GS结构域四个假定磷酸化位点上丝氨酸被丙氨酸取代的突变型ALK-4结合不佳。这些研究不仅阐明了Smad7对激活素信号传导的反调节功能,还表明激活素I型受体的磷酸化参与了Smad7的抑制作用。

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