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中期因子(一种具有神经营养活性的新型肝素结合生长/分化因子)视黄酸反应性增强子的定位与特性分析

Mapping and characterization of a retinoic acid-responsive enhancer of midkine, a novel heparin-binding growth/differentiation factor with neurotrophic activity.

作者信息

Matsubara S, Take M, Pedraza C, Muramatsu T

机构信息

Department of Biochemistry, Faculty of Medicine, Kagoshima University.

出版信息

J Biochem. 1994 Jun;115(6):1088-96. doi: 10.1093/oxfordjournals.jbchem.a124462.

Abstract

MK is a gene that is activated by retinoic acid in embryonal carcinoma (EC) cells and is expressed temporarily during the mid-gestation period of mouse embryogenesis. Midkine, the product of the gene is a novel heparin-binding growth/differentiation factor with neurite outgrowth and neurotrophic activities. The regulatory DNA element in the retinoic acid-induced expression of the MK gene has been investigated. The 1.9 kb 5'-flanking region of the MK gene can mediate retinoic acid-responsive gene expression in F9 and HM-1 EC cells. Analysis of this region by deletion mutagenesis in F9 EC cells shows that there is a retinoic acid-responsive enhancer (designated as REM1) around 900 bp upstream from the transcription start site. This enhancer is composed of two sequence elements, which are located between -1006 and -895 and between -901 and -794. The core element of the upstream region (-971 to -955), whose deletion abolished the retinoic acid responsiveness, contained a sequence highly homologous to a binding site for retinoic acid receptors. Binding of a retinoic acid receptor heterodimer to this core element was verified by gel shift assay. Thus, retinoic acid and the receptor complex can directly induce the expression of a growth/differentiation factor gene.

摘要

MK是一种在胚胎癌细胞中被视黄酸激活的基因,在小鼠胚胎发育的中期妊娠阶段暂时表达。该基因的产物中期因子是一种新型的肝素结合生长/分化因子,具有神经突生长和神经营养活性。人们已经对MK基因视黄酸诱导表达中的调控DNA元件进行了研究。MK基因1.9 kb的5'侧翼区域可介导F9和HM-1胚胎癌细胞中的视黄酸反应性基因表达。在F9胚胎癌细胞中通过缺失诱变对该区域进行分析表明,在转录起始位点上游约900 bp处存在一个视黄酸反应性增强子(命名为REM1)。该增强子由两个序列元件组成,分别位于-1006至-895以及-901至-794之间。上游区域的核心元件(-971至-955)缺失后消除了视黄酸反应性,其中包含一个与视黄酸受体结合位点高度同源的序列。通过凝胶迁移试验验证了视黄酸受体异二聚体与该核心元件的结合。因此,视黄酸和受体复合物可直接诱导生长/分化因子基因的表达。

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