The Human ICAM-2 Promoter is Endothelial Cell-specific in Vitro and in Vivo and Contains Critical Sp1 and GATA Binding Sites

塔塔盒子 报告基因 发起人 内皮干细胞 基因 转录因子 分子生物学 抄写(语言学) 细胞生物学 生物 基因表达 结合位点 体外 遗传学 哲学 语言学
作者
Peter J. Cowan,Denise Tsang,Christopher M. Pedic,Lucy R. Abbott,Trixie A. Shinkel,Anthony J.F. d’Apice,Martin J. Pearse
出处
期刊:Journal of Biological Chemistry [Elsevier BV]
卷期号:273 (19): 11737-11744 被引量:78
标识
DOI:10.1074/jbc.273.19.11737
摘要

The expression of intercellular adhesion molecule 2 (ICAM-2) in adult tissues is restricted to vascular endothelial cells and megakaryocytes. We have previously shown that the endothelial-specific in vivo activity of the human ICAM-2 promoter is contained within a small (0.33-kilobase (kbp)) 5′-flanking region of the gene. Here we describe the in vitrocharacterization of this region. The ICAM-2 promoter is TATA-less, and transcription in endothelial cells initiates at four sites. Reporter gene expression directed by the promoter was 125-fold greater than vector alone in bovine aortic endothelial cells but less than 2-fold vector alone in non-endothelial (COS) cells, confirming that specificity in vivo was paralleled in vitro. The addition of 2.7 kbp of 5′-flanking region to the 0.33-kbp fragment had no effect on promoter activity or specificity. The mutation of an Sp1 motif centered at base pair −194 or an eight-base pair palindrome at −268 each reduced promoter activity by 70%. Mutation of GATA motifs at −145 and −53 reduced promoter activity by 78 and 61%, respectively. Specific binding of bovine aortic endothelial cells nuclear proteins to the Sp1 and GATA sites was demonstrated by gel shift analysis. Promoter activity in COS cells was transactivated 3–4-fold by overexpression of GATA-2. The results presented here suggest that transcription from the ICAM-2 promoter in endothelial cells is regulated by the interplay of several positive-acting factors and provide the basis for further analysis of endothelial-specific gene expression.
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