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蛋白激酶CK2的调节性β亚基介导四聚体CK2复合物的形成。

The regulatory beta subunit of protein kinase CK2 mediates formation of tetrameric CK2 complexes.

作者信息

Graham K C, Litchfield D W

机构信息

Department of Biochemistry, Health Sciences Centre, University of Western Ontario, London, Ontario N6A 5C1, Canada.

出版信息

J Biol Chem. 2000 Feb 18;275(7):5003-10. doi: 10.1074/jbc.275.7.5003.

DOI:10.1074/jbc.275.7.5003
PMID:10671540
Abstract

Protein kinase CK2 is a tetrameric enzyme composed of two catalytic (alpha and/or alpha') subunits and two regulatory (beta) subunits. Because CK2beta is synthesized in excess of CK2alpha, we hypothesized that formation of CK2beta homodimers precedes the incorporation of the catalytic subunits of CK2 into complexes. To test this hypothesis, we cotransfected cells with two epitope-tagged variants of CK2beta. The results of these cotransfection studies demonstrate that interactions between two CK2beta subunits take place in the absence of CK2alpha. Together with results from previous biosynthetic labeling studies, these results suggest that formation of CK2beta homodimers occurs before incorporation of catalytic subunits of CK2 into CK2 complexes. We also cotransfected Cos-7 cells with a deletion fragment of CK2beta (i.e. Myc-beta1-166) together with full-length hemagglutinin (HA)-tagged CK2beta and/or CK2alpha'. Although complexes between Myc-beta1-166 and HA-beta were readily detected, we obtained no evidence of direct interactions between Myc-beta1-166 and HA-CK2alpha'. These results suggest that residues within the N-terminal 166 amino acids of CK2beta are sufficient for interactions between CK2beta subunits, whereas the C-terminal domain of CK2beta is required for complex formation with the catalytic subunits of CK2. Finally, we observed that expression of full-length HA-beta promotes phosphorylation of Myc-beta1-166 by HA-CK2alpha'.

摘要

蛋白激酶CK2是一种四聚体酶,由两个催化(α和/或α')亚基和两个调节(β)亚基组成。由于CK2β的合成量超过CK2α,我们推测CK2β同二聚体的形成先于CK2催化亚基掺入复合物中。为了验证这一假设,我们用两种带有表位标签的CK2β变体共转染细胞。这些共转染研究结果表明,在没有CK2α的情况下,两个CK2β亚基之间会发生相互作用。与之前生物合成标记研究的结果一起,这些结果表明CK2β同二聚体的形成发生在CK2催化亚基掺入CK2复合物之前。我们还用CK2β的缺失片段(即Myc-β1-166)与全长血凝素(HA)标签的CK2β和/或CK2α'共转染Cos-7细胞。虽然很容易检测到Myc-β1-166与HA-β之间的复合物,但我们没有获得Myc-β1-166与HA-CK2α'之间直接相互作用的证据。这些结果表明,CK2β N端166个氨基酸内的残基足以实现CK2β亚基之间的相互作用,而CK2β的C端结构域是与CK2催化亚基形成复合物所必需的。最后,我们观察到全长HA-β的表达促进了HA-CK2α'对Myc-β1-166的磷酸化作用。

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