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促黄体生成激素释放激素分泌神经元细胞系GT1-1中的类固醇结合与代谢

Steroid binding and metabolism in the luteinizing hormone-releasing hormone-producing neuronal cell line GT1-1.

作者信息

Poletti A, Melcangi R C, Negri-Cesi P, Maggi R, Martini L

机构信息

Institute of Endocrinology, University of Milan, Italy.

出版信息

Endocrinology. 1994 Dec;135(6):2623-8. doi: 10.1210/endo.135.6.7988451.

DOI:10.1210/endo.135.6.7988451
PMID:7988451
Abstract

LHRH synthesis and release are modulated in vivo by gonadal steroids. Although immunocytochemical and autoradiographic studies failed to detect appreciable amounts of estrogen or androgen receptor in LHRH-producing neurons, the recent finding that the promoter region of the LHRH gene contains several steroid hormone-responsive elements indicates a possible direct effect of sex steroids on these specialized neurons. The immortalized LHRH-producing neuronal cell line, GT1, which became recently available, may allow the study of LHRH dynamics. The presence of specific binding sites for estrogen and androgens as well as the presence of the two major enzymatic pathways involved in modulation of androgen action (the 5 alpha-reductase/3 alpha-hydroxysteroid dehydrogenase and the aromatase) have been studied in the GT1-1 clone. High affinity, low capacity binding sites for [3H]estradiol (Kd, 0.11 nM; binding capacity, 6.2 fmol/mg protein) and for a ligand of the androgen receptor, [3H]R1881 (Kd, 0.054 nM; binding capacity, 9.58 fmol/mg protein), have been identified in this cell line. A 2-fold induction of androgen-binding sites has been observed after 3 days of treatment of GT1-1 cells with estradiol (1 microM), indicating that the estradiol binding is probably linked to a functional estrogen receptor. Aromatase and 5 alpha-reductase/3 alpha-hydroxysteroid dehydrogenase activities have been also tested in GT1-1 cells. Under the culture conditions adopted, no detectable aromatization of [1 beta 3H]delta 4-androstenedione to estrone was observed using the tritiated water method. On the other hand, GT1-1 cells efficiently converted testosterone into dihydrotestosterone and subsequently into 5 alpha-androstan-3 alpha,17 beta-diol. In conclusion, GT1-1 cells possess several elements of the machinery through which sex steroids may influence LHRH dynamics.

摘要

促性腺激素释放激素(LHRH)的合成与释放受性腺甾体激素在体内的调节。尽管免疫细胞化学和放射自显影研究未能在产生LHRH的神经元中检测到可观数量的雌激素或雄激素受体,但最近发现LHRH基因的启动子区域包含几个甾体激素反应元件,这表明性甾体激素可能对这些特殊神经元有直接作用。最近获得的永生化产生LHRH的神经元细胞系GT1,可能有助于研究LHRH的动态变化。在GT1-1克隆中研究了雌激素和雄激素的特异性结合位点以及参与雄激素作用调节的两条主要酶促途径(5α-还原酶/3α-羟基类固醇脱氢酶和芳香化酶)的存在情况。在该细胞系中已鉴定出对[3H]雌二醇具有高亲和力、低容量的结合位点(解离常数Kd为0.11 nM;结合容量为6.2 fmol/mg蛋白质)以及对雄激素受体配体[3H]R1881具有高亲和力、低容量的结合位点(解离常数Kd为0.054 nM;结合容量为9.58 fmol/mg蛋白质)。在用雌二醇(1 μM)处理GT1-1细胞3天后,观察到雄激素结合位点增加了2倍,这表明雌二醇结合可能与功能性雌激素受体有关。还在GT1-1细胞中测试了芳香化酶和5α-还原酶/3α-羟基类固醇脱氢酶的活性。在所采用的培养条件下,使用氚水法未观察到[1β3H]δ4-雄烯二酮向雌酮的可检测芳香化作用。另一方面,GT1-1细胞能有效地将睾酮转化为二氢睾酮,随后再转化为5α-雄烷-3α,17β-二醇。总之,GT1-1细胞具有性甾体激素可能影响LHRH动态变化的几种机制要素。

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