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首页> 外文期刊>American Journal of Physiology >Cooperative effect of E2 and FGF2 on lactotroph proliferation triggered by signaling initiated at the plasma membrane
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Cooperative effect of E2 and FGF2 on lactotroph proliferation triggered by signaling initiated at the plasma membrane

机译:E2和FGF2对由质膜启动的信号触发的乳化营养增生的协同作用

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摘要

In the present work, we investigated the effect of 17β-estradiol (E2) and basic fibroblast growth factor 2 (FGF2) on the lactotroph cell-proliferative response and the related membrane-initiated signaling pathway. Anterior pituitary mixed-cell cultures of random, cycling 3-mo-old female rats were treated with 10 nM E2, E2 membrane-impermeable conjugated BSA (E2-BSA), PPT (ERα agonist), and DPN (ERβ agonist) alone or combined with FGF2 (10 ng/ml) for 30 min or 4 h. Although our results showed that the uptake of BrdU into the nucleus of lactotrophs was not modified by E2 or FGF2 alone, a significant increase in the lactotroph uptake of BrdU was observed after E2/FGF2 coincubation, with this effect being mimicked by PPT/FGF2. These proliferative effects were blocked by ICI 182,780 or PD-98059. The involvement of membrane ER in the proliferative response of prolactin cells induced by the steroid and FGF2 coincubation was confirmed using E2-BSA, and the association between ERα and FGF receptor was observed after E2/FGF2 treatment by immunoprecipitation. A significant increase in the ERK1/2 expression was noted after E2, E2-BSA, PPT, and FGF2 alone, which was more noticeable after E2-BSA/FGF2, E2/FGF2, or PPT/FGF2 treatments. This study provides evidence that E2 and FGF2 exert a cooperative effect on the lactotroph proliferation principally by signaling initiated at the plasma membrane triggering a genomic effect mediated by MEK/ERK1/2, a common signaling pathway, that finally regulates the lactotroph population, thus contributing to pituitary plasticity.
机译:在目前的工作中,我们研究了17β-雌二醇(E2)和碱性成纤维细胞生长因子2(FGF2)对乳酸菌的细胞增殖反应和相关的膜启动信号通路的影响。单独或单独用10 nM E2,不透E2膜的共轭BSA(E2-BSA),PPT(ERα激动剂)和DPN(ERβ激动剂)处理随机,循环的3个月大的雌性大鼠的垂体前叶混合细胞培养物。与FGF2(10 ng / ml)混合30分钟或4小时。尽管我们的研究结果表明,单独使用E2或FGF2并不能改变BrdU摄取到乳酸菌核中,但是在E2 / FGF2共孵育后,BrdU摄取的乳酸菌却显着增加,而PPT / FGF2可以模仿这种效应。这些增殖作用被ICI 182,780或PD-98059阻止。使用E2-BSA证实了膜ER参与类固醇和FGF2共孵育诱导的催乳素细胞的增殖反应,并且在通过免疫沉淀处理E2 / FGF2后观察到ERα和FGF受体之间的关联。单独使用E2,E2-BSA,PPT和FGF2后,ERK1 / 2表达显着增加,在使用E2-BSA / FGF2,E2 / FGF2或PPT / FGF2处理后,ERK1 / 2表达显着增加。这项研究提供了证据,证明E2和FGF2主要通过质膜上的信号触发由MEK / ERK1 / 2介导的基因组效应(一种常见的信号传导途径)最终对乳酸菌的种群进行调节,从而对乳酸菌的增殖发挥协同作用。垂体可塑性

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