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应激诱导的小鼠蛋白mSTI1。热休克蛋白结合域的特性及不同激酶的体外磷酸化作用。

Stress-inducible, murine protein mSTI1. Characterization of binding domains for heat shock proteins and in vitro phosphorylation by different kinases.

作者信息

Lässle M, Blatch G L, Kundra V, Takatori T, Zetter B R

机构信息

Department of Cell Biology and Surgery, Harvard Medical School and Children's Hospital, Boston, Massachusetts 02115, USA.

出版信息

J Biol Chem. 1997 Jan 17;272(3):1876-84. doi: 10.1074/jbc.272.3.1876.

DOI:10.1074/jbc.272.3.1876
PMID:8999875
Abstract

We have recently isolated the cDNA for the murine homologue of the stress-inducible phosphoprotein STI1 (also known as IEF SSP 3521 or p60). STI1 was previously shown to be 2-fold up-regulated in MRC-5 fibroblasts upon viral transformation and to exist in a macromolecular complex with heat shock proteins of the HSP 70 and 90 families. By peptide-sequencing we have identified the two heat shock proteins that bind to murine STI1 (mSTI1) as HSC 70 and HSP 84/86. We describe two separate binding regions within mSTI1 for the two heat shock proteins. In the presence of cell extracts, the N-terminal region of mSTI1 binds preferentially to HSC 70, whereas the C-terminal portion of the molecule promotes the binding of HSP 84/86. Heat treatment caused a strong induction of mSTI1 message without affecting the steady-state level of the protein significantly. In addition, heat treatment led to changes in the isoform-composition of mSTI1. pp70(s6k), pp90(rsk), and mitogen-activated protein kinase-activated protein kinase 2 were tested as possible STI1 kinases in vitro using recombinant mSTI1 as a substrate: only pp90(rsk) was able to phosphorylate recombinant mSTI1. In vitro kinase assays using casein kinase II suggest serine 189 to be a likely phosphorylation site in mSTI1.

摘要

我们最近分离出了应激诱导磷蛋白STI1(也称为IEF SSP 3521或p60)的小鼠同源物的cDNA。先前已证明,STI1在病毒转化后的MRC-5成纤维细胞中上调了2倍,并与HSP 70和90家族的热休克蛋白存在于大分子复合物中。通过肽测序,我们确定了与小鼠STI1(mSTI1)结合的两种热休克蛋白为HSC 70和HSP 84/86。我们描述了mSTI1内两个热休克蛋白的两个独立结合区域。在细胞提取物存在的情况下,mSTI1的N端区域优先与HSC 70结合,而分子的C端部分促进HSP 84/86的结合。热处理强烈诱导了mSTI1的信息,但对蛋白质的稳态水平没有显著影响。此外,热处理导致mSTI1的同工型组成发生变化。使用重组mSTI1作为底物,在体外测试了pp70(s6k)、pp90(rsk)和丝裂原活化蛋白激酶激活的蛋白激酶2作为可能的STI1激酶:只有pp90(rsk)能够磷酸化重组mSTI1。使用酪蛋白激酶II的体外激酶测定表明丝氨酸189可能是mSTI1中的磷酸化位点。

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