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DNA复制许可因子微小染色体维持蛋白7对表皮生长因子受体、c-Met和血小板衍生生长因子受体的RNA剪接至关重要。

The DNA replication licensing factor miniature chromosome maintenance 7 is essential for RNA splicing of epidermal growth factor receptor, c-Met, and platelet-derived growth factor receptor.

作者信息

Chen Zhang-Hui, Yu Yan P, Michalopoulos George, Nelson Joel, Luo Jian-Hua

机构信息

From the Departments of Pathology and.

Urology, University of Pittsburgh School of Medicine, Pittsburgh, Pennsylvania 15261.

出版信息

J Biol Chem. 2015 Jan 16;290(3):1404-11. doi: 10.1074/jbc.M114.622761. Epub 2014 Nov 25.

Abstract

Miniature chromosome maintenance 7 (MCM7) is an essential component of DNA replication licensing complex. Recent studies indicate that MCM7 is amplified and overexpressed in a variety of human malignancies. In this report, we show that MCM7 binds SF3B3. The binding motif is located in the N terminus (amino acids 221-248) of MCM7. Knockdown of MCM7 or SF3B3 significantly increased unspliced RNA of epidermal growth factor receptor, platelet-derived growth factor receptor, and c-Met. A dramatic drop of reporter gene expression of the oxytocin exon 1-intron-exon 2-EGFP construct was also identified in SF3B3 and MCM7 knockdown PC3 and DU145 cells. The MCM7 or SF3B3 depleted cell extract failed to splice reporter RNA in in vitro RNA splicing analyses. Knockdown of SF3B3 and MCM7 leads to an increase of cell death of both PC3 and DU145 cells. Such cell death induction is partially rescued by expressing spliced c-Met. To our knowledge, this is the first report suggesting that MCM7 is a critical RNA splicing factor, thus giving significant new insight into the oncogenic activity of this protein.

摘要

微小染色体维持蛋白7(MCM7)是DNA复制许可复合物的重要组成部分。最近的研究表明,MCM7在多种人类恶性肿瘤中发生扩增并过表达。在本报告中,我们发现MCM7与SF3B3结合。结合基序位于MCM7的N端(氨基酸221 - 248)。敲低MCM7或SF3B3可显著增加表皮生长因子受体、血小板衍生生长因子受体和c-Met的未剪接RNA。在敲低SF3B3和MCM7的PC3和DU145细胞中,还发现催产素外显子1-内含子-外显子2-EGFP构建体的报告基因表达显著下降。在体外RNA剪接分析中,耗尽MCM7或SF3B3的细胞提取物无法剪接报告RNA。敲低SF3B3和MCM7会导致PC3和DU145细胞的细胞死亡增加。通过表达剪接的c-Met可部分挽救这种细胞死亡诱导。据我们所知,这是首次报道表明MCM7是一种关键的RNA剪接因子,从而为该蛋白的致癌活性提供了重要的新见解。

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