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催乳素诱导的信号转导和转录激活因子(STAT)蛋白与α2-巨球蛋白(α2M)启动子的白细胞介素-6反应元件(IL-6RE)的结合及激活:与大鼠卵巢中α2M表达的关系

Prolactin-induced activation and binding of stat proteins to the IL-6RE of the alpha 2-macroglobulin (alpha 2M) promoter: relation to the expression of alpha 2M in the rat ovary.

作者信息

Russell D L, Norman R L, Dajee M, Liu X, Hennighausen L, Richards J S

机构信息

Department of Cell Biology, Baylor College of Medicine, Houston, Texas 77030, USA.

出版信息

Biol Reprod. 1996 Nov;55(5):1029-38. doi: 10.1095/biolreprod55.5.1029.

Abstract

Cellular signaling events by which prolactin (PRL) might regulate gene expression were analyzed in rat ovarian tissues. Whole cell extracts (WCE) were prepared from ovaries of pregnant rats (Days 4, 7, 9-11, 15, 17, and 21) and of hormonally primed (estradiol and FSH) hypophysectomized (H) immature rats before, or 15 min to 24 h after, acute administration of PRL (10 micrograms, i.v.). The DNA binding activity in the WCE was analyzed by electrophoretic mobility shift assays using the alpha 2-macroglobulin (alpha 2M) promoter interleukin (IL)-6 response element (IL-6RE) known to confer PRL and IL-6 inducibility to transgenes in target cells, including cultures of luteinized granulosa cells. Injections of PRL stimulated the appearance of a specific binding activity in ovarian extracts of H rats and in corpora lutea and interstitial extracts of pregnant rats from Days 4-9 of pregnancy. The presence of this protein/DNA complex was transient. The greater amount of binding was observed in luteinized tissue and interstitial tissue compared to follicles; and the binding activity contained specific tyrosine phosphorylated Stat (signal transduction and activators of transcription) factors identified by specific antibodies as acute phase response factor (APRF or Stat 3) and mammary gland factor (MGF, or Stat 5 [a and b]). In contrast to the transient activation and appearance of these factors in response to acute PRL treatment as administered to H rats or to pulsatile PRL release as occurs in early pregnancy, elevated levels of the same activated Stat factors were observed in WCE of CL and interstitial tissue prepared at mid-gestation (Days 10-17) when endogenous release of rat placental lactogen (rPL) is chronically elevated in serum. During this period, administration of additional exogenous PRL did not stimulate further activation (binding) of the Stat factors. During luteal regression (Day 21 of gestation) no binding was observed in the absence of PRL, and the response to PRL was markedly diminished despite the constitutive presence of Stat proteins and the Janus kinase that phosphorylates and activates these factors. Elevated binding of these factors to the IL-6RE of the alpha 2M promoter was associated with the expression of alpha 2M mRNA in luteinized granulosa cells and corpora lutea, indicating that activation of Stat factors is one mechanism by which PRL/rPL transactivates the alpha 2M gene in the tissue.

摘要

在大鼠卵巢组织中分析了催乳素(PRL)可能调节基因表达的细胞信号转导事件。从怀孕大鼠(第4、7、9 - 11、15、17和21天)以及经激素预处理(雌二醇和促卵泡激素)的垂体切除(H)未成熟大鼠的卵巢中制备全细胞提取物(WCE),这些未成熟大鼠在静脉注射PRL(10微克)之前、或注射后15分钟至24小时取材。使用α2 - 巨球蛋白(α2M)启动子白细胞介素(IL)- 6反应元件(IL - 6RE)通过电泳迁移率变动分析来分析WCE中的DNA结合活性,已知该元件可使转基因在包括黄体化颗粒细胞培养物在内的靶细胞中具有PRL和IL - 6诱导性。注射PRL刺激了H大鼠卵巢提取物以及妊娠第4 - 9天怀孕大鼠黄体和间质提取物中出现特异性结合活性。这种蛋白质/DNA复合物的存在是短暂的。与卵泡相比,在黄体化组织和间质组织中观察到更多的结合;并且结合活性包含通过特异性抗体鉴定为急性期反应因子(APRF或Stat 3)和乳腺因子(MGF,或Stat 5 [a和b])的特异性酪氨酸磷酸化Stat(信号转导和转录激活因子)。与给H大鼠急性注射PRL或妊娠早期出现的脉冲式PRL释放所引起的这些因子的短暂激活和出现相反,在妊娠中期(第10 - 17天)制备的CL和间质组织的WCE中观察到相同激活的Stat因子水平升高,此时大鼠胎盘催乳素(rPL)的内源性血清释放长期升高。在此期间,额外给予外源性PRL并未刺激Stat因子的进一步激活(结合)。在黄体退化期间(妊娠第21天),在没有PRL的情况下未观察到结合,并且尽管Stat蛋白和磷酸化并激活这些因子的Janus激酶持续存在,但对PRL的反应明显减弱。这些因子与α2M启动子的IL - 6RE的结合增加与黄体化颗粒细胞和黄体中α2M mRNA的表达相关,表明Stat因子的激活是PRL/rPL在组织中转录激活α2M基因的一种机制。

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