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首页> 外文期刊>Molecular human reproduction. >Progesterone inhibition of functional leptin receptor mRNA expression in human endometrium.
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Progesterone inhibition of functional leptin receptor mRNA expression in human endometrium.

机译:孕酮抑制人子宫内膜中功能性瘦素受体mRNA的表达。

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摘要

Leptin is secreted by adipocytes and regulates appetite through interaction with hypothalamic leptin receptors (OB-R). Leptin is involved in the stimulation of reproductive functions, and local expression of leptin and OB-R in the ovary, oocyte, embryo, and placenta might play a role in early development. The mRNA and protein of the long form leptin receptor (OB-R(L)) but not of leptin are expressed in the human endometrium and the abundance of OB-R mRNA expression varies during the menstrual cycle with a peak in the early secretory phase. We examined the steroidal regulation of OB-R(L) mRNA expression. Northern blot analyses showed that in organ-cultured proliferative endometrial specimens, oestradiol (10(-9) and 10(-8) mol/l) had no acute effect on the OB-R(L) mRNA expression, whereas oestradiol plus progesterone (10(-8), 10(-7) and 10(-6) mol/l) or medroxyprogesterone acetate (10(-8) and 10(-7) mol/l) suppressed the expression by approximately 50%. This progestin-induced suppression was blocked by a concomitant addition of mifepristone. Additionally, incubation of endometrial specimens in the presence of leptin resulted in the phosphorylation of its intracellular target, STAT3 (signal transducer and activator of transcription 3). These results indicate that, in the human endometrium, progestins act via the progesterone receptors to suppress functional OB-R(L) mRNA expression, and may thereby alter the sensitivity of the endometrium to leptin.
机译:瘦素由脂肪细胞分泌,并通过与下丘脑瘦素受体(OB-R)相互作用调节食欲。瘦素参与生殖功能的刺激,瘦素和OB-R在卵巢,卵母细胞,胚胎和胎盘中的局部表达可能在早期发育中起作用。长型瘦素受体(OB-R(L))的mRNA和蛋白在人子宫内膜中表达,而瘦素不表达。在月经周期,OB-R mRNA的表达量发生变化,在早期分泌期达到峰值。 。我们检查了OB-R(L)mRNA表达的甾体调节。 Northern印迹分析表明,在器官培养的子宫内膜标本中,雌二醇(10(-9)和10(-8)mol / l)对OB-R(L)mRNA表达没有急性影响,而雌二醇加孕酮( 10(-8),10(-7)和10(-6)mol / l)或醋酸甲羟孕酮(10(-8)和10(-7)mol / l)抑制表达约50%。伴随添加米非司酮可阻止这种由孕激素引起的抑制作用。另外,在瘦素存在下孵育子宫内膜标本会导致其胞内靶标STAT3(信号转导子和转录激活子3)磷酸化。这些结果表明,在人子宫内膜中,孕激素通过孕酮受体起作用以抑制功能性OB-R(L)mRNA表达,从而可能改变子宫内膜对瘦素的敏感性。

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