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一种新型核锌指蛋白EZI增强了STAT3的核内滞留和反式激活作用。

A novel nuclear zinc finger protein EZI enhances nuclear retention and transactivation of STAT3.

作者信息

Nakayama Koh, Kim Kyung-Woon, Miyajima Atsushi

机构信息

Institute of Molecular and Cellular Biosciences, The University of Tokyo, Yayoi, Bunkyo-ku, Tokyo 113-0032, Japan.

出版信息

EMBO J. 2002 Nov 15;21(22):6174-84. doi: 10.1093/emboj/cdf596.

DOI:10.1093/emboj/cdf596
PMID:12426389
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC137188/
Abstract

A novel cDNA EZI isolated as an oncostatin M- inducible gene encoded a protein containing 12 C2H2-type zinc fingers. EZI was found to transactivate the promoters that are also responsive to STAT3 and activated the acute phase response element (APRE) synergistically with STAT3. Co-immunoprecipitation demonstrated the association of EZI with STAT3, which was mediated by the N-terminal region (1-183) of EZI. The EZI mutant lacking this region showed reduced transcriptional activity, indicating that EZI and STAT3 function cooperatively through physical interaction. While EZI predominantly localized in the nucleus and enhanced the nuclear localization of STAT3, the EZI mutant lacking 11 zinc finger motifs failed to translocate into the nucleus and also inhibited nuclear localization of STAT3 as well as STAT3-mediated transactivation. These results indicate that EZI is a novel nuclear zinc finger protein that augments STAT3 activity by keeping it in the nucleus.

摘要

一个作为制瘤素M诱导基因分离得到的新cDNA EZI编码一种含有12个C2H2型锌指的蛋白质。发现EZI可反式激活对STAT3也有反应的启动子,并与STAT3协同激活急性期反应元件(APRE)。免疫共沉淀显示EZI与STAT3相互关联,这是由EZI的N端区域(1 - 183)介导的。缺失该区域的EZI突变体显示转录活性降低,表明EZI和STAT3通过物理相互作用协同发挥功能。虽然EZI主要定位于细胞核并增强STAT3的核定位,但缺失11个锌指基序的EZI突变体无法转运到细胞核中,并且还抑制STAT3的核定位以及STAT3介导的反式激活。这些结果表明EZI是一种新型核锌指蛋白,通过将STAT3保留在细胞核中来增强其活性。

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