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人类血型糖蛋白C基因启动子区域的结构及组织特异性

Structure of the promoter region and tissue specificity of the human glycophorin C gene.

作者信息

Le Van Kim C, Colin Y, Mitjavila M T, Clerget M, Dubart A, Nakazawa M, Vainchenker W, Cartron J P

机构信息

Institut National de la Santé et de la Recherche Médicale Unité U76, Institut National de Transfusion Sanguine, Paris, France.

出版信息

J Biol Chem. 1989 Dec 5;264(34):20407-14.

PMID:2584223
Abstract

Glycophorin C (GPC) is an integral membrane protein of human erythrocytes which plays an important role in regulating the deformability and mechanical stability of red cells. Recently, the structural gene for this glycoprotein has been cloned (Colin, Y., Le Van Kim, C., Tsapis, A., Clerget, M., d'Auriol, L., London, J., Galibert, F., and Cartron, J. P. (1989) J. Biol. Chem. 264, 3773-3780), and we have now determined the sequence of the 1050 base pairs of DNA preceding the transcription initiation site mapped in erythroid cells. This region contains different potential regulatory cis-acting elements found in a variety of eukaryotic promoters (TATA box, CAAT box, Sp1-binding site) as well as sequences present in the promoter and enhancer regions of genes specific for the erythroid lineage (CACCC box and NF-E1-binding site). Northern blot analysis and immunological studies indicate that the GPC gene is expressed in a large number of cells and tissues. However, the level of transcription as well as the glycosylation of the mature GPC differ in erythroid and nonerythroid cells. Primer extension analysis and mapping of the 5' end GPC mRNA by the polymerase chain reaction indicate that different transcription sites are utilized for the expression of the GPC gene in erythroid and nonerythroid tissues and cell lines.

摘要

血型糖蛋白C(GPC)是人类红细胞的一种整合膜蛋白,在调节红细胞的可变形性和机械稳定性方面发挥着重要作用。最近,这种糖蛋白的结构基因已被克隆(科林,Y.,勒万·金,C.,察皮斯,A.,克莱热,M.,奥里奥尔,L.,伦敦,J.,加利贝尔,F.,和卡特隆,J.P.(1989年)《生物化学杂志》264,3773 - 3780),我们现在已经确定了在红系细胞中定位的转录起始位点之前1050个碱基对的DNA序列。该区域包含在各种真核启动子中发现的不同潜在调控顺式作用元件(TATA盒、CAAT盒、Sp1结合位点)以及红系谱系特异性基因的启动子和增强子区域中存在的序列(CACCC盒和NF - E1结合位点)。Northern印迹分析和免疫学研究表明,GPC基因在大量细胞和组织中表达。然而,红系和非红系细胞中成熟GPC的转录水平以及糖基化情况有所不同。引物延伸分析和通过聚合酶链反应对GPC mRNA 5'端的定位表明,在红系和非红系组织及细胞系中,GPC基因的表达利用了不同的转录位点。

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