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人类阿黑皮素原基因启动子的调控元件

Regulatory elements of the human proopiomelanocortin gene promoter.

作者信息

Kraus J, Buchfelder M, Höllt V

机构信息

Department of Physiology, University of Munich, Germany.

出版信息

DNA Cell Biol. 1993 Jul-Aug;12(6):527-36. doi: 10.1089/dna.1993.12.527.

DOI:10.1089/dna.1993.12.527
PMID:8329120
Abstract

Proopiomelanocortin (POMC) is expressed predominantly in the corticotrophic cells of the pituitary. Regulatory sequences required for the expression of the human (h) POMC gene were investigated using transient expression of hPOMC-CAT fusion genes in pituitary and nonpituitary cells in combination with DNase I footprint and gel retardation assays. Gene transfer experiments revealed that the hPOMC promoter is more efficiently transcribed in AtT-20 pituitary cells than in HeLa cells. Using deletion analysis, negative regulatory elements between nucleotides -676 and -414 and positive regulatory elements between nucleotides -414 and -93 could be identified. When placed in front of the heterologous thymidine kinase (tk) promoter, nucleotides -414/-223 enhance transcription in AtT-20 cells and in primary cultures of human pituitary tumor cells, but not in various nonpituitary cell lines. In contrast, a -112/-93 element enhances transcription of the tk promoter in all cells tested. DNase I footprint analysis revealed five sites protected by nuclear extracts obtained from AtT-20 cells within nucleotides -414 and -83 of the hPOMC promoter region. In contrast, only one of these sites (between nucleotides -115 and -83) was protected by nuclear extracts from HeLa cells. Gel mobility-shift experiments revealed that an oligonucleotide comprising nucleotides -112/-93 binds a novel nuclear protein. This protein may contribute to the non-cell type-specific expression of the hPOMC gene outside the pituitary, whereas at least five transcription factors seem to be required for high basal transcription of the gene in corticotrophic cells.

摘要

阿黑皮素原(POMC)主要在垂体的促肾上腺皮质激素细胞中表达。利用hPOMC-CAT融合基因在垂体和非垂体细胞中的瞬时表达,并结合DNA酶I足迹分析和凝胶阻滞试验,研究了人(h)POMC基因表达所需的调控序列。基因转移实验表明,hPOMC启动子在AtT-20垂体细胞中的转录效率高于HeLa细胞。通过缺失分析,可以鉴定出核苷酸-676至-414之间的负调控元件和核苷酸-414至-93之间的正调控元件。当置于异源胸苷激酶(tk)启动子之前时,核苷酸-414/-223可增强AtT-20细胞和人垂体肿瘤细胞原代培养物中的转录,但在各种非垂体细胞系中则不然。相比之下,-112/-93元件可增强tk启动子在所有测试细胞中的转录。DNA酶I足迹分析显示,在hPOMC启动子区域的核苷酸-414和-83内,有五个位点受到AtT-20细胞获得的核提取物的保护。相比之下,HeLa细胞核提取物仅保护这些位点中的一个(核苷酸-115和-83之间)。凝胶迁移率变动实验表明,包含核苷酸-112/-93的寡核苷酸可结合一种新的核蛋白。这种蛋白质可能有助于hPOMC基因在垂体外的非细胞类型特异性表达,而该基因在促肾上腺皮质激素细胞中的高基础转录似乎至少需要五种转录因子。

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