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瘦素受体激活可增加人滋养层细胞中 Sam68 的酪氨酸磷酸化和表达。

Leptin receptor activation increases Sam68 tyrosine phosphorylation and expression in human trophoblastic cells.

机构信息

Department of Clinical Biochemistry, Virgen Macarena University Hospital, University of Seville, Av Dr Fedriani 3, Seville 41071, Spain.

出版信息

Mol Cell Endocrinol. 2011 Jan 30;332(1-2):221-7. doi: 10.1016/j.mce.2010.10.014. Epub 2010 Oct 28.

DOI:10.1016/j.mce.2010.10.014
PMID:21035519
Abstract

Leptin is produced in placenta where it has been found to be an important autocrine signal for trophoblastic growth during pregnancy, promoting antiapoptotic and trophic effects. Leptin receptor is present in trophoblastic cells and leptin may fully activate signaling. We have previously implicated the RNA-binding protein Sam68 in leptin signal transduction in immune cells. In the present work, we have studied the possible role of Sam68 in leptin receptor signaling in trophoblastic cells (JEG-3 cells). Leptin dose-dependently stimulated Sam68 phosphorylation in JEG-3 cells, as assessed by immunoprecipitation and immunoblot with anti-phosphotyrosine antibodies. As previously observed in other systems, tyrosine phosphorylation of Sam68 in response to leptin inhibits its RNA binding capacity. Besides, leptin stimulation dose-dependently increases Sam68 expression in JEG-3 cells, as assessed by quantitative PCR. Consistently, the amount of Sam68 protein is increased after 24h of leptin stimulation of trophoblastic cells. In order to study the possible role of Sam68 on leptin receptor synthesis, we employed antisense strategy to knockdown the expression of Sam68. We have found that a decrease in Sam68 expression leads to a decrease in leptin receptor amount in JEG-3 cells, as assessed both by quantitative PCR and immunoblot. These results strongly suggest the participation of Sam68 in leptin receptor signaling in human trophoblastic cells, and therefore, Sam68 may mediate some of the leptin effects in placenta.

摘要

瘦素在胎盘组织中产生,已被发现是妊娠期间滋养细胞生长的重要自分泌信号,促进抗凋亡和滋养作用。瘦素受体存在于滋养细胞中,瘦素可能完全激活信号。我们之前已经表明 RNA 结合蛋白 Sam68 在免疫细胞中的瘦素信号转导中起作用。在本工作中,我们研究了 Sam68 在滋养细胞(JEG-3 细胞)中瘦素受体信号转导中的可能作用。瘦素以剂量依赖的方式刺激 JEG-3 细胞中的 Sam68 磷酸化,如通过免疫沉淀和用抗磷酸酪氨酸抗体进行免疫印迹所评估的。如在其他系统中先前观察到的,瘦素刺激导致 Sam68 的酪氨酸磷酸化抑制其 RNA 结合能力。此外,如通过定量 PCR 所评估的,瘦素刺激以剂量依赖的方式增加 JEG-3 细胞中的 Sam68 表达。一致地,在滋养细胞接受瘦素刺激 24 小时后,Sam68 蛋白的量增加。为了研究 Sam68 对瘦素受体合成的可能作用,我们采用了反义策略来敲低 Sam68 的表达。我们发现,Sam68 表达的降低导致 JEG-3 细胞中的瘦素受体数量减少,如通过定量 PCR 和免疫印迹所评估的。这些结果强烈表明 Sam68 参与了人滋养细胞中的瘦素受体信号转导,因此,Sam68 可能介导胎盘内一些瘦素的作用。

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