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人类还原型叶酸载体基因的基础启动子受一个GC框和一个环磷酸腺苷反应元件/激活蛋白-1样元件调控。组织特异性基因表达的基础。

The basal promoters for the human reduced folate carrier gene are regulated by a GC-box and a cAMP-response element/AP-1-like element. Basis for tissue-specific gene expression.

作者信息

Whetstine J R, Matherly L H

机构信息

Department of Pharmacology, Wayne State University School of Medicine, Detroit, Michigan 48201, USA.

出版信息

J Biol Chem. 2001 Mar 2;276(9):6350-8. doi: 10.1074/jbc.M008074200. Epub 2000 Nov 14.

DOI:10.1074/jbc.M008074200
PMID:11078737
Abstract

Our laboratory previously identified two functional promoters (designated A and B) for the human reduced folate carrier (hRFC) gene that result in hRFC transcripts with differing 5'-untranslated regions. By transiently transfecting HT1080 and HepG2 cells with a series of 5' and 3' deletions in the hRFC-B and -A promoters, the minimal promoters were localized within 46 and 47 base pairs, respectively. Gel mobility shift assays with the hRFC-B basal promoter region revealed specific DNA-protein complexes involving a highly conserved GC-box and Sp1 or Sp3. In Drosophila SL2 cells, both Sp1 and the long Sp3 isoform potently transactivated the hRFC-B basal promoter; however, the short Sp3 isoforms were transcriptionally inert and resulted in a potent inhibition of Sp1 transactivation. For the hRFC-A basal promoter, a CRE/AP-1-like element was bound by the bZip superfamily of DNA-binding proteins. Cell-specific DNA-protein complexes were identified for hRFC-A (CREB-1 and c-Jun in HT1080 cells; CREB-1 and ATF-1 in HepG2 cells). When the GC-box and CRE/AP-1-like elements were mutated, a 60--90% decrease in promoter activity was observed in both cell lines. These results identify the critical regulatory regions for the hRFC basal promoters and stress the functional importance of the Sp and bZip families of transcription factors in regulating hRFC expression.

摘要

我们实验室先前鉴定出人类还原型叶酸载体(hRFC)基因的两个功能性启动子(分别命名为A和B),它们导致hRFC转录本具有不同的5'-非翻译区。通过用hRFC-B和-A启动子的一系列5'和3'缺失片段瞬时转染HT1080和HepG2细胞,最小启动子分别定位在46和47个碱基对内。用hRFC-B基础启动子区域进行凝胶迁移率变动分析,揭示了涉及高度保守的GC盒以及Sp1或Sp3的特异性DNA-蛋白质复合物。在果蝇SL2细胞中,Sp1和长的Sp3异构体均能有效激活hRFC-B基础启动子;然而,短的Sp3异构体在转录上无活性,并导致对Sp1反式激活的有效抑制。对于hRFC-A基础启动子,一个CRE/AP-1样元件被DNA结合蛋白的bZip超家族所结合。鉴定出了hRFC-A的细胞特异性DNA-蛋白质复合物(HT1080细胞中的CREB-1和c-Jun;HepG2细胞中的CREB-1和ATF-1)。当GC盒和CRE/AP-1样元件发生突变时,在两种细胞系中均观察到启动子活性下降60%-90%。这些结果确定了hRFC基础启动子的关键调控区域,并强调了Sp和bZip转录因子家族在调节hRFC表达中的功能重要性。

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