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钙调蛋白激酶I的亚型特异性激活及结构多样性

Isoform-specific activation and structural diversity of calmodulin kinase I.

作者信息

Naito Y, Watanabe Y, Yokokura H, Sugita R, Nishio M, Hidaka H

机构信息

Department of Pharmacology, Nagoya University School of Medicine, Showa-ku, Nagoya 466, Japan.

出版信息

J Biol Chem. 1997 Dec 19;272(51):32704-8. doi: 10.1074/jbc.272.51.32704.

DOI:10.1074/jbc.272.51.32704
PMID:9405489
Abstract

We earlier confirmed that there are isoforms of Ca2+/calmodulin (CaM)-dependent protein kinase I (CaM kinase I) (CaM kinase Ibeta1 and Igamma) beside CaM kinase Ialpha by cDNA cloning (Yokokura, H., Terada, O., Naito, Y., and Hidaka, H. (1997) Biochim. Biophys. Acta 1338, 8-12). Here, we demonstrate the existence of an isoform-specific activation mechanism of CaM kinase I and alternative splicing specifically regulating CaM kinase I (CaM kinase Ibeta2) in the central nervous system. To cast light on isoform structure-enzyme activity relationships, CaM kinase Ibeta1, Ibeta2, and Ialpha were expressed separately using a baculovirus/Sf9 cell expression system. The novel CaM kinase Ibeta2 isoform demonstrated similar catalytic activity to those of CaM kinase Ibeta1 and Ialpha. Interestingly, CaM kinase Ibeta1 and Ibeta2 both can activate CaM kinase Ialpha activity via phosphorylation at Thr177. Reverse transcribed-polymerase chain reaction analysis showed that CaM kinase Ibeta2 is dominant in the cerebrum and cerebellum, whereas CaM kinase Ibeta1 is present in peripheral tissues such as liver, heart, lung, kidney, spleen, and testis. CaM kinase Ibeta2 was also detected with an anti-CaM kinase Ibeta2 antibody in PC12 cells. The results indicate that alternative splicing is a means for tissue-specific expression of CaM kinase Ibeta. Thus the Thr177 residue of CaM kinase Ialpha is phosphorylated by not only CaM kinase kinase but also CaM kinase Ibeta for activation of the enzyme.

摘要

我们之前通过cDNA克隆(Yokokura, H., Terada, O., Naito, Y., and Hidaka, H. (1997) Biochim. Biophys. Acta 1338, 8 - 12)证实,除了钙调蛋白激酶Iα(CaM激酶Iα)之外,还存在钙调蛋白激酶I(CaM激酶I)的亚型(CaM激酶Iβ1和Iγ)。在此,我们证明了CaM激酶I存在亚型特异性激活机制,以及在中枢神经系统中特异性调节CaM激酶I(CaM激酶Iβ2)的可变剪接。为了阐明亚型结构与酶活性的关系,使用杆状病毒/Sf9细胞表达系统分别表达了CaM激酶Iβ1、Iβ2和Iα。新型的CaM激酶Iβ2亚型表现出与CaM激酶Iβ1和Iα相似的催化活性。有趣的是,CaM激酶Iβ1和Iβ2都可以通过在苏氨酸177处的磷酸化激活CaM激酶Iα的活性。逆转录-聚合酶链反应分析表明,CaM激酶Iβ2在大脑和小脑中占主导地位,而CaM激酶Iβ1存在于肝脏、心脏、肺、肾脏、脾脏和睾丸等外周组织中。在PC12细胞中也用抗CaM激酶Iβ2抗体检测到了CaM激酶Iβ2。结果表明,可变剪接是CaM激酶Iβ组织特异性表达的一种方式。因此,CaM激酶Iα的苏氨酸177残基不仅被CaM激酶激酶磷酸化,也被CaM激酶Iβ磷酸化以激活该酶。

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