首页> 美国卫生研究院文献>Aging (Albany NY) >Long non-coding RNA ANRIL alleviates H2O2-induced injury by up-regulating microRNA-21 in human lens epithelial cells
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Long non-coding RNA ANRIL alleviates H2O2-induced injury by up-regulating microRNA-21 in human lens epithelial cells

机译:长非编码RNA ANRIL通过上调人晶状体上皮细胞中的microRNA-21减轻H2O2诱导的损伤

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摘要

The accurate role of ANRIL in cataract is poorly understood. We aimed to reveal the effects of ANRIL on H O -treated HLECs, SRA01/04, as well as the regulatory mechanisms. Oxidative stress model of HLECs was induced by H O . Cell injury was evaluated according to cell proliferation, apoptosis and DNA damage using CCK-8 assay/flow cytometry and TUNEL assays/γH2AX staining. Expressions of ANRIL and miR-21 in HLECs were determined by RT-qPCR. The effects of miR-21, miR-34a and miR-122-5p inhibition as well as AMPK and β-catenin on HLECs with ANRIL overexpression and H O stimulation were analyzed. experiment was performed via RT-qPCR. H O repressed proliferation and induced apoptosis or DNA damage in HLECs. Those alterations induced by H O were attenuated by ANRIL overexpression. MiR-21 was positively regulated by ANRIL, and both of them were repressed in H O -induced HLECs and cataract patient tissues. Inhibition of miR-21 but not miR-34a or miR-122-5p reversed the effects of ANRIL on H O -treated HLECs. Phosphorylation of AMPK and expression of β-catenin were increased by ANRIL via regulating miR-21. AMPK and β-catenin affected beneficial function of ANRIL-miR-21 axis.
机译:人们对ANRIL在白内障中的确切作用了解甚少。我们旨在揭示ANRIL对H O处理的HLEC,SRA01 / 04以及调控机制的影响。 H O诱导HLECs的氧化应激模型。根据细胞增殖,凋亡和DNA损伤,使用CCK-8分析/流式细胞术和TUNEL分析/γH2AX染色评估细胞损伤。通过RT-qPCR确定HLEC中ANRIL和miR-21的表达。分析了miR-21,miR-34a和miR-122-5p抑制以及AMPK和β-catenin对具有ANRIL过表达和H O刺激的HLEC的影响。通过RT-qPCR进行实验。 H O抑制HLEC中的增殖并诱导凋亡或DNA损伤。 H O诱导的那些改变被ANRIL过表达所减弱。 MiR-21受到ANRIL的正调控,并且在HO诱导的HLEC和白内障患者组织中均被抑制。抑制miR-21而不抑制miR-34a或miR-122-5p可以逆转ANRIL对H O处理的HLEC的作用。 ANRIL通过调节miR-21增强AMPK的磷酸化和β-catenin的表达。 AMPK和β-catenin影响ANRIL-miR-21轴的有益功能。

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