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多胺与蛋白激酶CK2调节亚基的一个自主结构域结合会诱导全酶发生构象变化。这是激酶刺激的一个推测作用。

Binding of polyamines to an autonomous domain of the regulatory subunit of protein kinase CK2 induces a conformational change in the holoenzyme. A proposed role for the kinase stimulation.

作者信息

Leroy D, Heriché J K, Filhol O, Chambaz E M, Cochet C

机构信息

Laboratoire de Biochimie des Régulations Cellulaires Endocrines, Département de Biologie Moléculaire et Structurale, INSERM Unité 244, CEA Grenoble, 17 rue des Martyrs, F-38054 Grenoble Cedex 9, France.

出版信息

J Biol Chem. 1997 Aug 15;272(33):20820-7. doi: 10.1074/jbc.272.33.20820.

DOI:10.1074/jbc.272.33.20820
PMID:9252407
Abstract

The means by which the cell regulates protein kinase CK2 remain obscure. However, natural polyamines, cellular compounds required for cell proliferation, have been reported to strongly stimulate CK2-mediated phosphorylation of a number of substrates. Using spermine analogs, we have shown that polyamines directly interact with the CK2 beta subunit, and the chemical features of the highly acidic binding site (Asp51-Tyr80) have been determined. In the present study, we show that the isolated beta subunit region extending from residue Asp51 to Pro110 exhibits a specific and efficient polyamine binding activity similar to that of the entire beta subunit. Moreover, the replacement of Glu60, Glu61, and Glu63 of the beta subunit by 3 alanine residues leads to a loss of the spermine-induced stimulation of CK2 activity which correlates with a decrease in spermine binding affinity. Thermal stability studies indicate that the binding of spermine induces a 4 degrees C decrease of the Tm value for the holoenzyme. This was confirmed by circular dichroism analyses, which show that the 6 degrees C negative shift of the CK2 Tm value provoked by spermine binding, reflects a conformational change in the kinase. Together, these observations strongly suggest that this newly defined polyamine-binding domain is involved in the intrasteric regulation of CK2 activity.

摘要

细胞调节蛋白激酶CK2的方式仍不清楚。然而,据报道,天然多胺这种细胞增殖所需的细胞化合物能强烈刺激CK2介导的多种底物的磷酸化。利用精胺类似物,我们已经表明多胺直接与CK2β亚基相互作用,并且已经确定了高酸性结合位点(Asp51-Tyr80)的化学特征。在本研究中,我们表明,从Asp51残基延伸至Pro110的分离的β亚基区域表现出与整个β亚基相似的特异性和高效的多胺结合活性。此外,将β亚基的Glu60、Glu61和Glu63替换为3个丙氨酸残基会导致精胺诱导的CK2活性刺激丧失,这与精胺结合亲和力的降低相关。热稳定性研究表明,精胺的结合导致全酶的Tm值降低4℃。圆二色性分析证实了这一点,该分析表明,精胺结合引起的CK2 Tm值6℃的负向移动反映了激酶的构象变化。总之,这些观察结果强烈表明,这个新定义的多胺结合结构域参与了CK2活性的空间内调节。

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