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HSD17B1表达增强了低活性雌酮刺激的雌激素信号传导,这在体内由雌激素反应元件驱动的报告基因得以证明。

HSD17B1 expression enhances estrogen signaling stimulated by the low active estrone, evidenced by an estrogen responsive element-driven reporter gene in vivo.

作者信息

Järvensivu Päivi, Saloniemi-Heinonen Taija, Awosanya Michael, Koskimies Pasi, Saarinen Niina, Poutanen Matti

机构信息

Department of Physiology, University of Turku, Kiinamyllynkatu 10, FIN-20520 Turku, Finland.

Forendo Pharma Ltd., Itäinen Pitkäkatu 4, FIN-20520 Turku, Finland.

出版信息

Chem Biol Interact. 2015 Jun 5;234:126-34. doi: 10.1016/j.cbi.2015.01.008. Epub 2015 Jan 21.

DOI:10.1016/j.cbi.2015.01.008
PMID:25617485
Abstract

Hydroxysteroid (17beta) dehydrogenase 1 (HSD17B1) belongs to a family of short-chain-dehydrogenases. The enzyme utilizes NAD(P) and NAD(P)H as cofactors, and catalyzes the reversible reaction between estrone (E1) and estradiol (E2) in vitro. Of these steroids, E1 presents with lower estrogenic activity, but is converted to highly active E2 by HSD17B1. HSD17B1 is expressed especially in tissues with a high E2-producing capacity such as human ovaries and placenta, but also in several peripheral estrogen target tissues in humans, and inhibiting the enzyme activity is, thus, considered a promising approach to treat estrogen-dependent diseases. By analyzing transgenic mice universally expressing human HSD17B1 and carrying estrogen-response element (ERE)-driven luciferase reporter gene (Bi-transgenic ERELuc-HSD17B1TG mice) we showed a markedly higher reporter gene activity in various peripheral tissues of these mice as compared with ERELuc mice, indicating enhanced estrogen response generated by human HSD17B1 expression. An increased response after E1 administration was also evident in the Bi-TG mice, indicated by the increased uterus growth response and by the higher ERELuc reporter gene activity in the uterus. Moreover, a HSD17B1 inhibitor significantly reduced E1-induced increase in the uterus weight and uterine epithelial proliferation in the Bi-TG mice. Also the E1-induced ERELuc activity in the inhibitor-treated uterus was reduced by the HSD17B1 inhibitor in immature mice ex vivo, as well as in the liver of adult mice. The data, thus, demonstrate the potential use of the Bi-TG mice as a preclinical in vivo model for screening the efficacy of HSD17B1 inhibitors. As compared with the existing models, the Bi-TG mice present with luciferase activity as an additional, easily quantitative endpoint for the estrogen action.

摘要

羟类固醇(17β)脱氢酶1(HSD17B1)属于短链脱氢酶家族。该酶利用NAD(P)和NAD(P)H作为辅助因子,在体外催化雌酮(E1)和雌二醇(E2)之间的可逆反应。在这些类固醇中,E1的雌激素活性较低,但可被HSD17B1转化为高活性的E2。HSD17B1尤其在具有高E2产生能力的组织中表达,如人类卵巢和胎盘,也在人类的一些外周雌激素靶组织中表达,因此,抑制该酶的活性被认为是治疗雌激素依赖性疾病的一种有前景的方法。通过分析普遍表达人类HSD17B1并携带雌激素反应元件(ERE)驱动的荧光素酶报告基因的转基因小鼠(双转基因ERELuc-HSD17B1TG小鼠),我们发现与ERELuc小鼠相比,这些小鼠的各种外周组织中报告基因活性明显更高,表明人类HSD17B1表达产生了增强的雌激素反应。双转基因小鼠在给予E1后反应增强也很明显,表现为子宫生长反应增加以及子宫中ERELuc报告基因活性更高。此外,一种HSD17B1抑制剂显著降低了双转基因小鼠中E1诱导的子宫重量增加和子宫上皮增殖。在未成熟小鼠的离体子宫以及成年小鼠的肝脏中,HSD17B1抑制剂也降低了抑制剂处理的子宫中E1诱导的ERELuc活性。因此,这些数据证明了双转基因小鼠作为筛选HSD17B1抑制剂疗效的临床前体内模型的潜在用途。与现有模型相比,双转基因小鼠具有荧光素酶活性,作为雌激素作用的另一个易于定量的终点。

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