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鉴定一种受白细胞介素-1调节的细胞质蛋白激酶,该激酶可使小热休克蛋白hsp27磷酸化。

Identification of a cytoplasmic protein kinase regulated by IL-1 that phosphorylates the small heat shock protein, hsp27.

作者信息

Guesdon F, Saklatvala J

机构信息

Cytokine Biochemistry Department, Strangeways Research Laboratory, Cambridge, United Kingdom.

出版信息

J Immunol. 1991 Nov 15;147(10):3402-7.

PMID:1940343
Abstract

IL-1 increases phosphorylation of the small heat shock protein (hsp27) in intact cells. This change was also shown both by introducing [gamma-32P]ATP and Mg2+ into MRC-5 fibroblasts permeabilized by LPC after stimulation by IL-1, and by adding the labeled ATP and Mg2+ to cell extracts. Hsp27 phosphorylated in permeabilized cells or cell extracts was shown by 2D electrophoresis to comprise the three forms seen in metabolically labeled cells, suggesting that the physiologically relevant kinase was acting on the substrate in vitro. Mixing of extracts of resting and IL-1-stimulated cells revealed that stimulated cells contained increased levels of kinase activity that phosphorylated substrate hsp27 in the extracts of resting cells. Existence of the activated kinase was confirmed by showing that extracts of IL-1-stimulated cells phosphorylated purified homogeneous hsp27 at a greater rate than those of resting cells. The kinase activity was maximal in cells stimulated with IL-1 for 5 to 10 min, but had declined to the resting level after stimulation for 40 min. Membrane and cytosolic fractions prepared from cell homogenates both contained hsp27 kinase, but the IL-1-dependent increase was associated with the cytosolic fraction. TNF-stimulated cells also contained increased hsp27 kinase activity in the cytosol. The evidence suggests that the cytosolic hsp27 kinase is responsible for the changes in hsp27 phosphorylation induced by the cytokines in intact cells.

摘要

白细胞介素-1(IL-1)可增加完整细胞中小分子热休克蛋白(hsp27)的磷酸化水平。在用IL-1刺激后,通过向经溶血卵磷脂(LPC)通透处理的MRC-5成纤维细胞中引入[γ-32P]ATP和Mg2+,以及向细胞提取物中添加标记的ATP和Mg2+,均证实了这一变化。二维电泳显示,通透细胞或细胞提取物中磷酸化的hsp27包含代谢标记细胞中所见的三种形式,这表明生理相关激酶在体外作用于底物。静止细胞和IL-1刺激细胞提取物的混合实验表明,刺激细胞中激酶活性水平升高,可使静止细胞提取物中的底物hsp27发生磷酸化。通过显示IL-1刺激细胞的提取物比静止细胞的提取物以更高的速率磷酸化纯化的均一hsp27,证实了活化激酶的存在。激酶活性在IL-1刺激5至10分钟的细胞中最高,但在刺激40分钟后已降至静止水平。从细胞匀浆制备的膜和胞质部分均含有hsp27激酶,但IL-1依赖性增加与胞质部分相关。肿瘤坏死因子(TNF)刺激的细胞胞质中hsp27激酶活性也增加。证据表明,胞质hsp27激酶负责细胞因子在完整细胞中诱导的hsp27磷酸化变化。

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