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Expression of Estrogen Receptor α 36 (ESR36) in the Hamster Ovary throughout the Estrous Cycle: Effects of Gonadotropins

机译:整个发情周期中仓鼠卵巢中雌激素受体α36(ESR36)的表达:促性腺激素的作用

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摘要

Estradiol-17β (E) plays an important role in ovarian follicular development. Evidence indicates that some of the effect of E is mediated by the transmembrane estrogen receptor. In this study, we examined the spatio-temporal expression of recently discovered ERα36 (ESR36), a splice variant of Esr1 and a receptor for non-genomic E signaling, in the hamster ovary during the estrous cycle and the role of gonadotropins and ovarian steroid hormones in ESR36 expression. ESR36 expression was high on estrus (D1∶0900 h) and declined precipitously by proestrus (D4∶0900 h) and remained low up to D4∶1600 h. Immunofluorescence findings corroborated immunoblot findings and revealed that ESR36 was expressed only in the cell membrane of both follicular and non-follicular cells, except the oocytes. Ovarian ESR36 was capable of binding to the E-affinity matrix, and have different molecular weight than that of the ESR1 or GPER. Hypophysectomy (Hx) resulted in a marked decline in ESR36 protein levels. FSH and LH, alone or combined, markedly upregulated ESR36 protein in Hx hamsters to the levels observed in D1 hamsters, but neither E nor P had any effect. Inhibition of the gonadotropin surge by phenobarbital treatment on D4∶1100 h attenuated ESR36 expression in D1∶0900 h ovaries, but the decline was restored by either FSH or LH replacement on D4 afternoon. This is the first report to show that ESR36, which is distinct from ESR1 or GPER is expressed in the plasma membrane of ovarian follicular and non-follicular cells, binds to E and its expression is regulated directly by the gonadotropins. In light of our previous findings, the results suggest that ovarian cells contain at least two distinct membrane estrogen receptors, such as GPER and ESR36, and strongly suggest for a non-genomic action of E regulating ovarian follicular functions.
机译:雌二醇17β(E)在卵巢卵泡发育中起重要作用。有证据表明,E的某些作用是由跨膜雌激素受体介导的。在这项研究中,我们检查了发情周期中仓鼠卵巢中最近发现的ERα36(ESR36),Esr1的剪接变体和非基因组E信号受体的时空表达以及促性腺激素和卵巢类固醇的作用ESR36表达中的激素。 ESR36在发情期(D1∶0900 h)表达高,而在发情期前(D4∶0900 h)急剧下降,在D4∶1600 h时仍低。免疫荧光结果证实了免疫印迹的发现,并揭示了ESR36仅在卵母细胞和非卵泡细胞的细胞膜中表达,除了卵母细胞。卵巢癌ESR36能够结合E-亲和基质,并且分子量不同于ESR1或GPER。垂体切除术(Hx)导致ESR36蛋白水平显着下降。单独或联合使用的FSH和LH将Hx仓鼠中的ESR36蛋白显着上调至D1仓鼠中观察到的水平,但E和P均无作用。苯巴比妥对D4∶1100h抑制促性腺激素激增使D1∶0900h卵巢的ESR36表达减弱,但在D4下午通过FSH或LH替代恢复了下降。这是第一个表明与ESR1或GPER不同的ESR36在卵巢滤泡和非滤泡细胞的质膜中表达,与E结合且其表达受促性腺激素直接调节的报告。根据我们先前的发现,结果表明卵巢细胞至少包含两种不同的膜雌激素受体,例如GPER和ESR36,并强烈暗示E调节卵巢卵泡功能的非基因作用。

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