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GATA转录因子对促红细胞生成素基因表达的负调控

Negative regulation of the erythropoietin gene expression by the GATA transcription factors.

作者信息

Imagawa S, Yamamoto M, Miura Y

机构信息

Department of Medicine, Jichi Medical School, Tochigi-ken, Japan.

出版信息

Blood. 1997 Feb 15;89(4):1430-9.

PMID:9028967
Abstract

We examined regulation of the human erythropoietin (Epo) gene through the GATA sequence in the Epo promoter and showed that Hep3B and HepG2 cells express human GATA-2 (hGATA-2) mRNA and protein. Nuclear extracts of QT6 cells transfected with hGATA-1, 2, or 3 transcription factors showed specific binding to the GATA element in the human Epo gene promoter by gel mobility shift assay. Transient transfection of Hep3B cells with hGATA-1, 2, or 3 showed that each of these transcription factors significantly decreased the level of expression of Epo mRNA as assessed by a competitive polymerase chain reaction. Transient transfection of Hep3B cells with hGATA-1, 2, and 3 and an Epo-reporter gene (growth hormone [GH]) construct showed significant inhibition of the Epo promoter. Antisense oligonucleotide for hGATA-2 transcription factor significantly increased the Epo protein in Hep3B cells under 1% O2 for 24 hours incubation. Furthermore, transient transfection of Hep3B cells with hGATA-1, 2, and 3 and an Epo-reporter gene (luciferase) construct also showed significant inhibition of the Epo promoter. However, transfection of the mutated GATA sequence of the Epo-luciferase gene with hGATA-1, 2, and 3 interfere with the inhibition of the Epo promoter. We conclude that the hGATA-1, 2, and 3 transcription factors specifically bind to the GATA element in the human Epo gene promoter and negatively regulate Epo gene expression.

摘要

我们通过促红细胞生成素(Epo)启动子中的GATA序列研究了人类促红细胞生成素基因的调控,结果表明Hep3B和HepG2细胞表达人类GATA-2(hGATA-2)mRNA和蛋白质。通过凝胶迁移率变动分析,用hGATA-1、2或3转录因子转染的QT6细胞的核提取物显示与人促红细胞生成素基因启动子中的GATA元件有特异性结合。用hGATA-1、2或3对Hep3B细胞进行瞬时转染,结果显示通过竞争性聚合酶链反应评估,这些转录因子中的每一种都显著降低了促红细胞生成素mRNA的表达水平。用hGATA-1、2和3以及促红细胞生成素报告基因(生长激素[GH])构建体对Hep3B细胞进行瞬时转染,结果显示促红细胞生成素启动子受到显著抑制。针对hGATA-2转录因子的反义寡核苷酸在1%氧气条件下孵育24小时后,显著增加了Hep3B细胞中的促红细胞生成素蛋白。此外,用hGATA-1、2和3以及促红细胞生成素报告基因(荧光素酶)构建体对Hep3B细胞进行瞬时转染,也显示促红细胞生成素启动子受到显著抑制。然而,用hGATA-1、2和3转染促红细胞生成素-荧光素酶基因的突变GATA序列会干扰对促红细胞生成素启动子的抑制作用。我们得出结论,hGATA-1、2和3转录因子与人促红细胞生成素基因启动子中的GATA元件特异性结合,并对促红细胞生成素基因表达起负调控作用。

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