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Ste20 样激酶(SLK)的活性通过同源二聚化增强。

Activity of the Ste20-like kinase, SLK, is enhanced by homodimerization.

机构信息

Department of Medicine, McGill University Health Centre, McGill University, Montreal, Quebec, Canada.

出版信息

Am J Physiol Renal Physiol. 2011 Sep;301(3):F554-64. doi: 10.1152/ajprenal.00062.2011. Epub 2011 Jun 15.

Abstract

The expression and activation of the Ste20-like kinase, SLK, is increased during renal development and recovery from ischemic acute renal failure. SLK promotes apoptosis, and during renal injury and repair, transcriptional induction or posttranscriptional control of SLK may, therefore, regulate cell survival. SLK contains protein interaction (coiled-coil) domains, suggesting that posttranslational homodimerization may also modulate SLK activity. We therefore expressed coiled-coil regions in the C-terminal domain of SLK as fusion proteins and demonstrated their homodimerization. By gel-filtration chromatography, endogenous and heterologously expressed SLK were detected in a macromolecular protein complex. To test the role of homodimerization in kinase activation, we constructed a fusion protein consisting of the SLK catalytic domain (amino acids 1-373) and a modified FK506 binding protein, Fv (Fv-SLK 1-373). Addition of AP20187 (an analog of FK506) enhanced the homodimerization of Fv-SLK 1-373. In an in vitro kinase assay, the dimeric Fv-SLK 1-373 displayed greater kinase activity than the monomeric form. In cells expressing Fv-SLK 1-373, homodimerization increased activation-specific phosphorylation of the proapoptotic kinases, c-Jun N-terminal kinase and p38 kinase. Compared with the monomer, dimeric Fv-SLK 1-373 enhanced the activation of a Bax promoter-luciferase reporter. Finally, expression of Fv-SLK 1-373 induced apoptosis, and the effect was increased by homodimerization. Thus the activity, downstream signaling, and functional effects of SLK are enhanced by dimerization of the kinase domain.

摘要

丝裂原活化蛋白激酶激酶样激酶(Ste20-like kinase,SLK)的表达和激活在肾发育和缺血性急性肾衰竭恢复过程中增加。SLK 促进细胞凋亡,因此,在肾损伤和修复过程中,SLK 的转录诱导或转录后控制可能调节细胞存活。SLK 含有蛋白相互作用(卷曲螺旋)结构域,表明翻译后同源二聚化也可能调节 SLK 活性。因此,我们将 SLK 羧基末端结构域中的卷曲螺旋区表达为融合蛋白,并证明了它们的同源二聚化。通过凝胶过滤层析,在内源和异源表达的 SLK 中检测到大分子蛋白复合物。为了测试同源二聚化在激酶激活中的作用,我们构建了一个由 SLK 催化结构域(氨基酸 1-373)和修饰的 FK506 结合蛋白 Fv(Fv-SLK 1-373)组成的融合蛋白。添加 AP20187(FK506 的类似物)增强了 Fv-SLK 1-373 的同源二聚化。在体外激酶测定中,二聚体 Fv-SLK 1-373 的激酶活性大于单体形式。在表达 Fv-SLK 1-373 的细胞中,同源二聚化增加了促凋亡激酶 c-Jun N 末端激酶和 p38 激酶的激活特异性磷酸化。与单体相比,二聚体 Fv-SLK 1-373 增强了 Bax 启动子-荧光素酶报告基因的激活。最后,表达 Fv-SLK 1-373 诱导细胞凋亡,并且同源二聚化增加了该效应。因此,激酶结构域的二聚化增强了 SLK 的活性、下游信号转导和功能效应。

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