晚期糖基化终产物干扰人卵巢颗粒细胞 KGN 中黄体生成素和卵泡刺激素的信号转导。
Advanced glycation end products interfere in luteinizing hormone and follicle stimulating hormone signaling in human granulosa KGN cells.
机构信息
1 Endocrinology Department, Hellenic Red Cross Hospital, Athens 11526, Greece.
2 Institute of Clinical Chemistry and Laboratory Medicine, Technische Universität Dresden, Dresden 01307, Germany.
出版信息
Exp Biol Med (Maywood). 2018 Jan;243(1):29-33. doi: 10.1177/1535370217731288. Epub 2017 Sep 15.
Advanced glycation end products accumulate in the ovarian granulosa-cell layer of women with polycystic ovarian syndrome. Taken that the MAPK/ERK-pathway is a key regulator of oocyte maturation and function, consisting the main pathway used by the gonadotrophic hormones (luteinizing hormone, follicle stimulating hormone) to control ovulation, the present study aims to assess advanced glycation end products' interference into luteinizing hormone-and follicle stimulating hormone-signaling via the MAPK/ERK-pathway in the human granulosa KGN cell line. KGN cells were treated with luteinizing hormone or follicle stimulating hormone in the absence or presence of human glycated albumin. The specific activation of the main components of the MAPK/ERK1/2-pathway (namely c-Raf, MEK and ERK1/2) was assessed. Treatment of KGN cells with an MEK1/2-inhibitor or a blocking anti-RAGE-antibody was also performed to shed further light on the mechanism of the involvement of advanced glycation end products in luteinizing hormone and/or follicle stimulating hormone-related signaling pathways. Luteinizing hormone treatment increased p-ERK1/2 levels in human granulosa cells, while the combined treatment of luteinizing hormone and human glycated albumin provoked a decrease of p-ERK1/2 levels. A similar reducing effect was also observed for the upstream molecule phospho-cRaf upon combined treatment, while treatment with an MEK-inhibitor confirmed that the phenomenon is MAPK/ERK-pathway-dependent. Similarly, follicle stimulating hormone treatment increased p-ERK1/2 and p-MEK1/2 levels, while the combined treatment of follicle stimulating hormone and human glycated albumin downregulated their levels. Advanced glycation end products reduce the luteinizing hormone- and follicle stimulating hormone-induced ERK1/2 activation that is critical for granulosa cell mitogenesis and proliferation. Inappropriate activation of ERK1/2 in granulosa cells may block the granulosa cell differentiation pathway and/or impair follicular responses to hormones, potentially leading to ovulation failure that characterizes polycystic ovarian syndrome.
晚期糖基化终产物在多囊卵巢综合征妇女的卵巢颗粒细胞层中积累。鉴于 MAPK/ERK 通路是卵母细胞成熟和功能的关键调节剂,是促性腺激素(黄体生成素、卵泡刺激素)用来控制排卵的主要途径,本研究旨在评估晚期糖基化终产物通过 MAPK/ERK 通路对人颗粒细胞 KGN 细胞系中黄体生成素和卵泡刺激素信号的干扰。用黄体生成素或卵泡刺激素处理 KGN 细胞,同时存在或不存在人糖化白蛋白。评估了 MAPK/ERK1/2 通路的主要成分(即 c-Raf、MEK 和 ERK1/2)的特异性激活。还进行了用 MEK1/2 抑制剂或阻断性抗 RAGE 抗体处理 KGN 细胞,以进一步阐明晚期糖基化终产物参与黄体生成素和/或卵泡刺激素相关信号通路的机制。黄体生成素处理增加了人颗粒细胞中的 p-ERK1/2 水平,而黄体生成素和人糖化白蛋白的联合处理则降低了 p-ERK1/2 水平。联合处理时,上游分子磷酸化 cRaf 也观察到类似的降低作用,而 MEK 抑制剂的处理证实了这一现象是 MAPK/ERK 通路依赖性的。同样,卵泡刺激素处理增加了 p-ERK1/2 和 p-MEK1/2 水平,而卵泡刺激素和人糖化白蛋白的联合处理则下调了它们的水平。晚期糖基化终产物降低了黄体生成素和卵泡刺激素诱导的 ERK1/2 激活,这对颗粒细胞有丝分裂和增殖至关重要。颗粒细胞中 ERK1/2 的异常激活可能会阻断颗粒细胞分化途径和/或损害卵泡对激素的反应,可能导致多囊卵巢综合征的排卵失败。
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