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雌二醇对脂氧素 A4 合酶启动子活性的调节:直接和间接机制的证据。

Estradiol regulation of lipocalin-type prostaglandin D synthase promoter activity: evidence for direct and indirect mechanisms.

机构信息

Laboratory of Neurobiology and Behavior, Rockefeller University, 1230 York Ave, New York, NY 10021, United States.

出版信息

Neurosci Lett. 2010 Apr 19;474(1):17-21. doi: 10.1016/j.neulet.2010.02.064. Epub 2010 Mar 1.

Abstract

In the CNS, lipocalin-type prostaglandin D synthase (L-PGDS) is predominantly a non-neuronal enzyme responsible for the production of PGD(2), an endogenous sleep promoting substance. We have previously demonstrated that estradiol differentially regulates L-PGDS transcript levels in the rodent brain. In hypothalamic nuclei, estradiol increases L-PGDS transcript expression, whereas in the ventrolateral preoptic area L-PGDS gene expression is reduced after estradiol treatment. In the present study, we have used an immortalized glioma cell line transfected with a L-PGDS reporter construct and estrogen receptor (ER) alpha and ERbeta expression plasmids to further elucidate the mechanisms underlying estradiol regulation of L-PGDS gene expression. We found that physiologically relevant concentrations of estradiol evoked an inverted U response in cells expressing ERalpha. The most effective concentration of estradiol (10(-11)M) increased the promoter activity 3-fold over baseline. Expression of ERbeta did not increase activity over control and when ERbeta was co-expressed with ERalpha there was a significant attenuation of the promoter activity. While ERalpha significantly increased L-PGDS promoter activity, our previous in vivo studies demonstrate a greater magnitude of change in L-PGDS gene expression in the presences of estradiol. This led us to ask whether estradiol is signaling via a paracrine factor released by the neighboring neurons. Conditioned media from estradiol treated neurons applied to the glioma cell line resulted in a significant 7-fold increase in L-PGDS promoter activity supporting the possibility that neuronal-glial interactions are involved in estradiol regulation of L-PGDS.

摘要

在中枢神经系统中,脂氧合酶型前列腺素 D 合酶(L-PGDS)主要是非神经元酶,负责产生 PGD(2),一种内源性促进睡眠的物质。我们之前已经证明,雌激素对啮齿动物大脑中的 L-PGDS 转录水平有差异调节作用。在下丘脑核中,雌激素增加 L-PGDS 转录表达,而在腹外侧视前区,雌激素处理后 L-PGDS 基因表达减少。在本研究中,我们使用转染了 L-PGDS 报告基因构建体和雌激素受体(ER)α和 ERβ表达质粒的永生化神经胶质瘤细胞系,进一步阐明了雌激素调节 L-PGDS 基因表达的机制。我们发现,生理相关浓度的雌激素在表达 ERα 的细胞中引起了倒 U 型反应。最有效的雌激素浓度(10(-11)M)使启动子活性比基线增加了 3 倍。ERβ的表达并没有增加活性超过对照,并且当 ERβ与 ERα共表达时,启动子活性显著减弱。虽然 ERα显著增加了 L-PGDS 启动子活性,但我们之前的体内研究表明,在存在雌激素的情况下,L-PGDS 基因表达的变化幅度更大。这促使我们询问雌激素是否通过相邻神经元释放的旁分泌因子进行信号传递。用雌激素处理的神经元的条件培养基应用于神经胶质瘤细胞系,导致 L-PGDS 启动子活性显著增加了 7 倍,支持神经元-神经胶质相互作用参与雌激素对 L-PGDS 的调节的可能性。

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