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雌二醇通过转录依赖性机制对促性腺激素释放激素-1神经元活动产生直接作用。

Direct action of estradiol on gonadotropin-releasing hormone-1 neuronal activity via a transcription-dependent mechanism.

作者信息

Temple Jennifer L, Laing Eric, Sunder Anushka, Wray Susan

机构信息

Cellular and Developmental Neurobiology Section, National Institute of Neurological Disorders and Stroke, National Institutes of Health, Bethesda, Maryland 20892, USA.

出版信息

J Neurosci. 2004 Jul 14;24(28):6326-33. doi: 10.1523/JNEUROSCI.1006-04.2004.

Abstract

Pulsatile secretion of gonadotropin-releasing hormone-1 (GnRH-1) is essential for reproduction. GnRH-1 induces gonadotropin release and is regulated by 17beta-estradiol (E2). Although a subpopulation of GnRH-1 neurons expresses estrogen receptor (ER) beta, it is unclear whether E2 acts directly on GnRH-1 neurons or indirectly through interneuronal connections. To test the hypothesis that E2 acts directly on GnRH-1 neurons to regulate neuronal activity, we used calcium imaging to monitor intracellular calcium oscillations in GnRH-1 neurons maintained in nasal explants. TTX was used to minimize synaptic input from other cells. Consistent with previous studies, TTX reduced the activity of individual GnRH-1 neurons to a basal level, while the population of cells maintained synchronized calcium oscillations. Exposure of GnRH-1 cells to TTX plus E2 increased the number of calcium peaks/cell, percentage of cells with > or =10 peaks, mean peak amplitude, and percentage of cells that contributed to each calcium pulse in explants maintained in vitro for 7 d (7 div) compared with TTX alone. These effects were induced within 30 min and were not mimicked by 17alpha-estradiol, E2 conjugated to BSA (which does not cross the plasma membrane), or seen at 21 div, when the percentage of GnRH-1 cells expressing ERbeta transcripts declines. In addition, these effects were inhibited by the ER antagonist ICI 182,780 and prevented by inhibition of gene transcription. These data suggest that, via ERbeta, E2 can rapidly act as a hormone-activated transcription complex and are the first to show that E2 directly increases GnRH-1 neuronal activity and synchronization.

摘要

促性腺激素释放激素-1(GnRH-1)的脉冲式分泌对生殖至关重要。GnRH-1诱导促性腺激素释放,并受17β-雌二醇(E2)调节。尽管GnRH-1神经元的一个亚群表达雌激素受体(ER)β,但尚不清楚E2是直接作用于GnRH-1神经元还是通过神经元间连接间接起作用。为了验证E2直接作用于GnRH-1神经元以调节神经元活动的假说,我们使用钙成像技术监测鼻外植体中GnRH-1神经元的细胞内钙振荡。使用河豚毒素(TTX)来尽量减少来自其他细胞的突触输入。与先前的研究一致,TTX将单个GnRH-1神经元的活性降低至基础水平,而细胞群体维持同步的钙振荡。与单独使用TTX相比,将GnRH-1细胞暴露于TTX加E2可增加体外培养7天(7日龄)的外植体中每个细胞的钙峰数量、具有≥10个峰的细胞百分比、平均峰幅度以及对每个钙脉冲有贡献的细胞百分比。这些效应在30分钟内诱导产生,17α-雌二醇、与牛血清白蛋白(BSA)结合的E2(其不能穿过质膜)不能模拟这些效应,并且在21日龄时未观察到这些效应,此时表达ERβ转录本的GnRH-1细胞百分比下降。此外,这些效应被ER拮抗剂ICI 182,780抑制,并因基因转录抑制而被阻止。这些数据表明,E2可通过ERβ迅速作为激素激活的转录复合物发挥作用,并且首次表明E2直接增加GnRH-1神经元活性和同步性。

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