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通过光亲和标记直接鉴定蛋白激酶酪蛋白激酶2调节亚基上的多胺结合结构域。

Direct identification of a polyamine binding domain on the regulatory subunit of the protein kinase casein kinase 2 by photoaffinity labeling.

作者信息

Leroy D, Schmid N, Behr J P, Filhol O, Pares S, Garin J, Bourgarit J J, Chambaz E M, Cochet C

机构信息

INSERM Unit 244, Departement de Biologie Molécularie et Structurale, Centre d'Etudes Nucléaires/Grenoble, France.

出版信息

J Biol Chem. 1995 Jul 21;270(29):17400-6. doi: 10.1074/jbc.270.29.17400.

DOI:10.1074/jbc.270.29.17400
PMID:7615545
Abstract

Phosphorylation of many protein substrates by the protein kinase casein kinase 2 (CK2) is stimulated severalfold in the presence of polyamines such as spermine. Previous experiments have shown that CK2 is a polyamine binding protein and that the regulatory beta subunit is required for this binding activity. To delineate the spermine binding site of CK2, we have applied a photoaffinity labeling method using a tritiated photoactivable analog of spermine, [3H]sperminediazonium. The photoaffinity labeled beta subunit was cleaved with cyanogen bromide, and two labeled peptides were separated by high performance liquid chromatography. The major one was the peptide T72EQAAEM78 and the minor one was a 22-amino acid peptide comprising residues Ile98 to Met119. Thr72 and His108 were identified as the labeled amino acids of the Thr72-Met78 and Ile98-Met119 peptides, respectively. In the same manner, we succeeded in determining the residue Leu220 as an alpha subunit residue covalently bound to the probe. The photoaffinity labeling method described here enabled the first elucidation, by direct microsequencing, of a polyamine binding site on CK2 for which we propose a provisional structural model. These observations suggest a possible mechanism for CK2 activation by polyamines at the molecular level.

摘要

在诸如精胺等多胺存在的情况下,蛋白激酶酪蛋白激酶2(CK2)对许多蛋白质底物的磷酸化作用会增强数倍。先前的实验表明,CK2是一种多胺结合蛋白,且这种结合活性需要调节性β亚基。为了描绘CK2的精胺结合位点,我们应用了一种光亲和标记方法,使用精胺的氚化光活化类似物[3H]精胺重氮盐。光亲和标记的β亚基用溴化氰裂解,两个标记的肽段通过高效液相色谱分离。主要的肽段是T72EQAAEM78,次要的是一个包含Ile98至Met119残基的22个氨基酸的肽段。Thr72和His108分别被鉴定为Thr72 - Met78和Ile98 - Met119肽段的标记氨基酸。同样,我们成功地确定Leu220残基是与探针共价结合的α亚基残基。这里描述的光亲和标记方法通过直接微测序首次阐明了CK2上的一个多胺结合位点,我们为此提出了一个初步的结构模型。这些观察结果提示了多胺在分子水平上激活CK2的一种可能机制。

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