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生长激素细胞中催乳素基因表达的抑制与位点特异性DNA甲基化相关。

Suppression of prolactin gene expression in GH cells correlates with site-specific DNA methylation.

作者信息

Zhang Z X, Kumar V, Rivera R T, Pasion S G, Chisholm J, Biswas D K

机构信息

Laboratory of Molecular Biology, Harvard School of Dental Medicine, Boston, MA 02115.

出版信息

DNA. 1989 Oct;8(8):605-13. doi: 10.1089/dna.1989.8.605.

DOI:10.1089/dna.1989.8.605
PMID:2480873
Abstract

Prolactin- (PRL) producing and nonproducing subclones of the GH line of (rat) pituitary tumor cells have been compared to elucidate the regulatory mechanisms of PRL gene expression. Particular emphasis was placed on delineating the molecular basis of the suppressed state of the PRL gene in the prolactin-nonproducing (PRL-) GH subclone (GH(1)2C1). We examined six methylatable cytosine residues (5, -CCGG- and 1, -GCGC-) within the 30-kb region of the PRL gene in these subclones. This analysis revealed that -CCGG-sequences of the transcribed region, and specifically, one in the fourth exon of the PRL gene, were heavily methylated in the PRL-, GH(1)2C1 cells. Furthermore, the inhibition of PRL gene expression in GH(1)2C1 was reversed by short-term treatment of the cells with a sublethal concentration of azacytidine (AzaC), an inhibitor of DNA methylation. The reversion of PRL gene expression by AzaC was correlated with the concurrent demethylation of the same -CCGG- sequences in the transcribed region of PRL gene. An inverse correlation between PRL gene expression and the level of methylation of the internal -C- residues in the specific -CCGG-sequence of the transcribed region of the PRL gene was demonstrated. The DNase I sensitivity of these regions of the PRL gene in PRL+, PRL-, and AzaC-treated cells was also consistent with an inverse relationship between methylation state, a higher order of structural modification, and gene expression.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

为阐明催乳素(PRL)基因表达的调控机制,对大鼠垂体肿瘤细胞GH系中产生PRL和不产生PRL的亚克隆进行了比较。特别着重于描绘PRL基因在不产生催乳素(PRL-)的GH亚克隆(GH(1)2C1)中受抑制状态的分子基础。我们检测了这些亚克隆中PRL基因30kb区域内的六个可甲基化胞嘧啶残基(5′-CCGG-和1′-GCGC-)。该分析显示,转录区域的-CCGG-序列,特别是PRL基因第四外显子中的一个,在PRL-的GH(1)2C1细胞中高度甲基化。此外,用亚致死浓度的阿扎胞苷(AzaC,一种DNA甲基化抑制剂)对细胞进行短期处理,可逆转GH(1)2C1中PRL基因表达的抑制。AzaC使PRL基因表达逆转与PRL基因转录区域中相同-CCGG-序列的同时去甲基化相关。PRL基因表达与PRL基因转录区域特定-CCGG-序列内部-C-残基的甲基化水平呈负相关。PRL+、PRL-和AzaC处理细胞中PRL基因这些区域的DNase I敏感性也与甲基化状态、更高阶结构修饰和基因表达之间的负相关关系一致。(摘要截短于250字)

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