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丙酮酸激酶红细胞特异性启动子的转录调控

Transcriptional regulation of the pyruvate kinase erythroid-specific promoter.

作者信息

Max-Audit I, Eleouet J F, Roméo P H

机构信息

Institut National de la Santé et de la Recherche Médicale U.91, Hôpital Henri Mondor, Créteil, France.

出版信息

J Biol Chem. 1993 Mar 15;268(8):5431-7.

PMID:8449904
Abstract

Mammal pyruvate kinases are encoded by two genes. The L gene produces the erythroid (R-PK) or the hepatic (L-PK) isozymes by the alternative use of two promoters. We report the characterization of the cis- and trans-acting elements involved in the tissue-specific activity of the L gene erythroid promoter. A R-PK DNA fragment extending from -870 to +54 relative to the cap site confers erythroid specificity to a reporter gene. Within this region, we define a minimal promoter (-62 to +54) that displays erythroid-specific activity and contains two DNA binding sites. One, located at -50, binds members of the CCACC/Sp1 family and the other, located at -20, binds the erythroid factor GATA-1. Although the -20 GATA binding site (AGATAA) is also a potential TFIID binding site, it does not bind TFIID. Furthermore, the substitution of this GATA binding site by a canonical TFIID binding site suppresses the promoter activity. Mutations and deletions of both sites indicate that only the association of CCACC/Sp1 and GATA binding sites can drive efficient and tissue-specific expression of this R-PK minimal promoter. Finally, by co-transfection experiments, we study the elements involved in the hGATA-1 transactivation of the R-PK promoter in HeLa cells.

摘要

哺乳动物丙酮酸激酶由两个基因编码。L基因通过交替使用两个启动子产生红系(R-PK)或肝系(L-PK)同工酶。我们报道了参与L基因红系启动子组织特异性活性的顺式和反式作用元件的特征。相对于帽位点,从-870延伸至+54的R-PK DNA片段赋予报告基因红系特异性。在该区域内,我们定义了一个最小启动子(-62至+54),其具有红系特异性活性并包含两个DNA结合位点。一个位于-50,结合CCACC/Sp1家族成员;另一个位于-20,结合红系因子GATA-1。尽管-20的GATA结合位点(AGATAA)也是潜在的TFIID结合位点,但它不结合TFIID。此外,用典型的TFIID结合位点替换该GATA结合位点会抑制启动子活性。两个位点的突变和缺失表明,只有CCACC/Sp1和GATA结合位点的结合才能驱动该R-PK最小启动子的高效和组织特异性表达。最后,通过共转染实验,我们研究了HeLa细胞中参与R-PK启动子hGATA-1反式激活的元件。

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