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p160类固醇受体辅激活因子2(SRC-2)调节小鼠子宫内膜功能,并调节不依赖孕酮和依赖孕酮的基因表达。

The p160 steroid receptor coactivator 2, SRC-2, regulates murine endometrial function and regulates progesterone-independent and -dependent gene expression.

作者信息

Jeong Jae-Wook, Lee Kevin Y, Han Sang Jun, Aronow Bruce J, Lydon John P, O'Malley Bert W, DeMayo Francesco J

机构信息

Department of Molecular and Cellular Biology, Baylor College of Medicine, Houston, Texas 77030, USA.

出版信息

Endocrinology. 2007 Sep;148(9):4238-50. doi: 10.1210/en.2007-0122. Epub 2007 Jun 7.

DOI:10.1210/en.2007-0122
PMID:17556502
Abstract

The role of the p160 steroid receptor coactivator 2 (SRC-2) in the regulation of uterine function and progesterone (P4) signaling was investigated by determining the expression pattern of SRC-2 in the murine uterus during pregnancy and the impact of SRC-2 ablation on uterine function and global uterine gene expression in response to progesterone. SRC-2 is expressed in the endometrial luminal and glandular epithelium from pregnancy d 0.5. SRC-2 is then expressed in the endometrial stroma on pregnancy d 2.5-3.5. Once the embryo is implanted, SRC-2 is expressed in the endometrial stromal cells in the secondary decidual zone. This compartmental expression of SRC-2 can be mimicked by treatment of ovariectomized mice with estrogen and P4. Ablation of SRC-2 in the uterus resulted in a significant reduction in the ability of the uterus to undergo a hormonally induced decidual reaction. Microarray analysis of RNA from uteri of wild-type and SRC-2(-/-) mice treated with vehicle or P4 showed that SRC-2 was involved in the ability of progesterone to repress specific genes. This microarray analysis also revealed that the uteri of SRC-2(-/-) mice showed alterations in genes involved in estrogen receptor, Wnt, and bone morphogenetic protein signaling. This analysis indicates that SRC-2 regulates uterine function by modulating the regulation of developmentally important signaling molecules and the ability of P4 to repress specific genes.

摘要

通过确定妊娠期间小鼠子宫中p160类固醇受体共激活因子2(SRC-2)的表达模式以及SRC-2基因敲除对子宫功能和子宫整体基因表达对孕酮反应的影响,研究了SRC-2在子宫功能调节和孕酮(P4)信号传导中的作用。从妊娠第0.5天开始,SRC-2在子宫内膜腔上皮和腺上皮中表达。然后在妊娠第2.5至3.5天,SRC-2在子宫内膜基质中表达。一旦胚胎着床,SRC-2就在次级蜕膜区的子宫内膜基质细胞中表达。用雌激素和P4处理去卵巢小鼠可模拟SRC-2的这种分区表达。子宫中SRC-2的基因敲除导致子宫对激素诱导的蜕膜反应能力显著降低。对用赋形剂或P4处理的野生型和SRC-2基因敲除(-/-)小鼠子宫的RNA进行微阵列分析表明,SRC-2参与孕酮抑制特定基因的能力。该微阵列分析还显示,SRC-2基因敲除(-/-)小鼠的子宫在涉及雌激素受体、Wnt和骨形态发生蛋白信号传导的基因方面出现改变。该分析表明,SRC-2通过调节发育重要信号分子的调控以及P4抑制特定基因的能力来调节子宫功能。

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