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孕激素对人乳腺癌细胞中雌激素受体信使核糖核酸的调控

Progestin regulation of estrogen receptor messenger RNA in human breast cancer cells.

作者信息

Alexander I E, Shine J, Sutherland R L

机构信息

Garvan Institute of Medical Research, St. Vincent's Hospital, Sydney, New South Wales, Australia.

出版信息

Mol Endocrinol. 1990 Jun;4(6):821-8. doi: 10.1210/mend-4-6-821.

DOI:10.1210/mend-4-6-821
PMID:2233741
Abstract

Progestin antagonism of estrogen action is thought to be due, at least in part, to progestin down-regulation of the estrogen receptor (ER). The molecular mechanisms subserving this effect, and the functional consequences in terms of target cell sensitivity to estrogens, are poorly understood. The present study was undertaken to address these issues with particular emphasis on progestin regulation of ER gene expression at the mRNA level. The T-47D human breast cancer cell line was treated with the synthetic progestin, ORG 2058, and the resultant changes in ER mRNA and ER levels determined by Northern analysis and radioligand binding, respectively. Treatment of T-47D cells with ORG 2058 resulted in rapid down-regulation of ER mRNA levels to a nadir of 35-40% of control by 6 h. This fall in ER mRNA levels was accompanied by a slower but more sustained fall in ER binding to a nadir of 20% of control at 24 h. Between 12 and 24 h ER mRNA levels recovered partially while ER ligand binding continued to fall. At 48 h both ER mRNA and ER concentrations remained depressed, although the latter to a greater extent. ER mRNA half-life was determined by [3H]uridine incorporation to be approximately 60 min and was unaffected by progestin treatment during the early rapid phase of ER mRNA down-regulation. These data demonstrate that progestins cause rapid down-regulation of the ER mRNA and suggest that during the early rapid phase of this effect, reduced transcription of the ER gene rather than altered ER mRNA half-life mediate this effect.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

孕激素对雌激素作用的拮抗作用至少部分被认为是由于孕激素使雌激素受体(ER)下调所致。关于这种作用的分子机制以及靶细胞对雌激素敏感性方面的功能后果,目前了解甚少。本研究旨在解决这些问题,特别关注孕激素在mRNA水平对ER基因表达的调控。用合成孕激素ORG 2058处理T - 47D人乳腺癌细胞系,分别通过Northern分析和放射性配体结合法测定ER mRNA和ER水平的变化。用ORG 2058处理T - 47D细胞导致ER mRNA水平迅速下调,至6小时时降至对照的35 - 40%的最低点。ER mRNA水平的这种下降伴随着ER结合的下降,速度较慢但更持久,至24小时时降至对照的20%的最低点。在12至24小时之间,ER mRNA水平部分恢复,而ER配体结合继续下降。在48小时时,ER mRNA和ER浓度均仍处于较低水平,尽管后者下降幅度更大。通过[3H]尿苷掺入法测定ER mRNA半衰期约为60分钟,在ER mRNA下调的早期快速阶段,孕激素处理对其无影响。这些数据表明,孕激素可导致ER mRNA迅速下调,并提示在这种作用的早期快速阶段,是ER基因转录减少而非ER mRNA半衰期改变介导了这种作用。(摘要截短至250字)

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