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黄嘉, 李芮冰, 王成彬. UPRmt改善乙醇诱导的肝细胞坏死性凋亡的分子机制研究[J]. 解放军医学院学报, 2023, 44(6): 700-707. DOI: 10.3969/j.issn.2095-5227.2023.06.020
引用本文: 黄嘉, 李芮冰, 王成彬. UPRmt改善乙醇诱导的肝细胞坏死性凋亡的分子机制研究[J]. 解放军医学院学报, 2023, 44(6): 700-707. DOI: 10.3969/j.issn.2095-5227.2023.06.020
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HUANG Jia, LI Ruibing, WANG Chengbin. Molecular mechanism of UPRmt in ameliorating alcohol-induced hepatocyte necroptosis[J]. ACADEMIC JOURNAL OF CHINESE PLA MEDICAL SCHOOL, 2023, 44(6): 700-707. DOI: 10.3969/j.issn.2095-5227.2023.06.020
Citation: HUANG Jia, LI Ruibing, WANG Chengbin. Molecular mechanism of UPRmt in ameliorating alcohol-induced hepatocyte necroptosis[J]. ACADEMIC JOURNAL OF CHINESE PLA MEDICAL SCHOOL, 2023, 44(6): 700-707. DOI: 10.3969/j.issn.2095-5227.2023.06.020
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UPRmt改善乙醇诱导的肝细胞坏死性凋亡的分子机制研究

Molecular mechanism of UPRmt in ameliorating alcohol-induced hepatocyte necroptosis

    摘要
  • 摘要:
      背景  坏死性凋亡作为一种新型程序性细胞死亡方式参与酒精性肝病的发生发展。线粒体未折叠的蛋白质反应(mitochondrial unfolded protein response, UPRmt)能够促进应激反应中细胞修复并改善线粒体网络的调控,探究乙醇诱导下肝细胞内UPRmt调控机制可能为酒精性肝病的临床治疗提供新的潜在靶点。
      目的  探讨UPRmt对乙醇诱导下肝细胞线粒体功能和坏死性凋亡的影响,及其在肝细胞线粒体网络中的作用机制。
      方法  利用正常小鼠肝细胞AML12构建正常对照组、乙醇组、UPRmt激活对照组、UPRmt激活乙醇组模型。经浓度250 mmol/L无水乙醇培养细胞构建乙醇组模型,通过造模前6 h给予10 μmol/L寡霉素A激活正常小鼠肝细胞UPRmt构建干预组。利用RT-PCR检测UPRmt、线粒体分裂和坏死性凋亡相关基因转录水平,荧光探针观察线粒体功能,蛋白质印迹法检测自噬相关蛋白表达水平。
      结果  乙醇诱导下UPRmt相关基因mtDNAj、CHOP、ATF5和炎症因子TNF-α、IL-6、Timp1转录水平升高,坏死性凋亡关键基因RIPK3、PGAM5表达增加(P<0.05)。荧光探针观察到乙醇诱导下线粒体膜电位显著下降,线粒体ROS产生量增多(P<0.05),蛋白免疫印迹结果显示乙醇诱导下肝细胞内线粒体自噬被抑制,线粒体分裂增加。寡霉素A干预增强细胞内UPRmt,从而改善乙醇诱导下炎症产生和氧化应激,维持线粒体正常功能,抑制肝细胞坏死性凋亡。
      结论  UPRmt通过减少细胞氧化应激、维持线粒体正常功能,从而缓解乙醇诱导的肝细胞坏死性凋亡和炎症损伤。

     

    Abstract:
      Background  Long-term alcohol consumption can cause serious liver damage. As a new programmed cell death mode, necroptosis is involved in the pathogenesis of alcoholic liver disease (ALD). Mitochondrial unfolded protein response (UPRmt) can promote cell recovery and improve mitochondrial network survival. Exploring the role of UPRmt in ALD may provide a new potential target for clinical practice.
      Objective  To investigate the effect of UPRmt on mitochondrial function and ethanol-induced hepatocyte necroptosis and supplement mechanisms of UPRmt in hepatocyte mitochondrial network.
      Methods  Four groups were constructed, including normal control group (NC), alcoholic liver disease group (ALD), UPRmt activation control group (NC + Omy), and UPRmt activation alcoholic liver disease group (ALD + Omy). ALD group was cultured in the completed culture medium with 250 mmol/L ethanol, and 10 μmol/L oligomycin A was added 6 hours before modeling to activate hepatocytes UPRmt. RT-PCR was used to detect key genes transcriptional levels of UPRmt, mitochondrial fission and necroptosis. Fluorescence probe was used to observe mitochondrial function. Western blotting was performed to detect the expression levels of mitophagy proteins, such as microtubule-associated protein 1 light chain 3 (LC3), P62 and Fundc1.
      Results  RT-PCR results showed that the transcription level of UPRmt related genes mtDNAj, CHOP, ATF5 and inflammatory factor TNF- α, IL-6 and Timp1 increased induced by alcohol, and the expression of key genes of necrotic apoptosis RIPK3 and PGAM5 also increased (P<0.05). The mitochondrial membrane potential significantly decreased while the production of mtROS increased in ALD model (P<0.05). Western blotting results showed reduced mitophagy and abnormal mitochondrial fission in ALD model. Oligomycin A intervention reversed these damages, threfore reducing inflammation and oxidative stress, maintaining the normal mitochondrial function, and inhibiting hepatocytes necroptosis.
      Conclusion  UPRmt alleviates alcohol-induced hepatocyte necroptosis by rescuing oxidative stress and mitochondrial dysfunction.

     

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