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Transcription factors regulate GPR91-mediated expression of VEGF in hypoxia-induced retinopathy

机译:转录因子调节VPR91介导的VEGF在缺氧诱导的视网膜病变中的表达

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Hypoxia is the most important factor in the pathogenesis of diabetic retinopathy (DR). Our previous studies demonstrated that G protein-coupled receptor 91(GPR91) participated in the regulation of vascular endothelial growth factor (VEGF) secretion in DR. The present study induced OIR model in newborn rats using exposure to alternating 24-hour episodes of 50% and 12% oxygen for 14 days. Treatment with GPR91 shRNA attenuated the retinal avascular area, abnormal neovascularization and pericyte loss. Western blot and qRT-PCR demonstrated that CoCl2 exposure promoted VEGF expression and secretion, activated the ERK1/2 signaling pathways and upregulated C/EBP and AP-1. Knockdown of GPR91 inhibited ERK1/2 activity. GPR91 siRNA transduction and the ERK1/2 inhibitor U0126 inhibited the increases in C/EBP β, C/EBP δ, c-Fos and HIF-1α. Luciferase reporter assays and a chromatin immunoprecipitation (ChIP) assay demonstrated that C/EBP β and c-Fos bound the functional transcriptional factor binding site in the region of the VEGF promoter, but not C/EBP δ. Knockdown of C/EBP β and c-Fos using RNAi reduced VEGF expression. Our data suggest that activation of the GPR91-ERK1/2-C/EBP β (c-Fos, HIF-1α) signaling pathway plays a tonic role in regulating VEGF transcription in rat retinal ganglion cells.
机译:缺氧是糖尿病视网膜病变(DR)发病机制最重要的因素。我们以前的研究表明,G蛋白偶联受体91(GPR91)参与了博士中血管内皮生长因子(VEGF)分泌的调节。本研究诱导新生大鼠的OIR模型,使用暴露于50%和12%氧的交替的24小时发作14天。用GPR91 ShRNA治疗减弱视网膜缺血面积,异常新生血管和细胞损失。蛋白质印迹和QRT-PCR证明了COCL2曝光促进了VEGF表达和分泌,活化了ERK1 / 2信号传导途径和上调的C / EBP和AP-1。 GPR91的敲低抑制ERK1 / 2活性。 GPR91 siRNA转导和ERK1 / 2抑制剂U0126抑制C / EBPβ,C /EBPδ,C-FOS和HIF-1α的增加。荧光素酶报告器测定和染色质免疫沉淀(芯片)测定证明C /EBPβ和C-FOS在VEGF启动子区域中结合功能性转录因子结合位点,但不是C /EBPδ。使用RNAI降低VEGF表达的C / EBPβ和C-FOS的敲低。我们的数据表明,GPR91-ERK1 / 2-C /EBPβ(C-FOS,HIF-1α)信号通路的激活在调节大鼠视网膜神经节细胞中的VEGF转录方面发挥了滋补作用。

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