Pan Pan, Chen Jie, Liu Xudong, Fan Junping, Zhang Dong, Zhao Weiguo, Xie Lixin, Su Longxiang
College of Pulmonary and Critical Care Medicine, Chinese PLA General Hospital, Beijing, China.
Department of Respiratory Medicine, Xiangya Hospital, Central South University, Changsha, Hunan Province, China.
Shock. 2021 Nov 1;56(5):773-781. doi: 10.1097/SHK.0000000000001835.
The incidence and mortality of acute respiratory distress syndrome (ARDS) are high, but the relevant mechanism for this disorder remains unclear. Autophagy plays an important role in the development of ARDS. The mitochondrial outer membrane protein FUNDC1 is involved in hypoxia-mediated mitochondrial autophagy, which may contribute to ARDS development. This study explored whether FUNDC1 regulates autophagy by inhibiting ROS-NLRP3 signaling to avoid apoptosis in the lung in a lipopolysaccharide-induced mouse model. In this study, FUNDC1 knockout mice were constructed, and a lipopolysaccharide-induced mouse model was generated. HE staining of pathological sections from the lung, wet/dry lung measurements, myeloperoxidase concentration/neutrophil counts in BALF and survival time of mice were examined to determine the effect of modeling. The release of cytokines (TNF-α, IL-1β, IL-6, and IL-10) in response to LPS in the BALF and plasma was assessed using ELISA. The effects of oxidative stress (malondialdehyde, superoxide dismutase, catalase, glutathione peroxidase) in lung tissue in response to LPS were detected by biochemical analysis. Oxidative stress damage was validated by iNOS staining, and apoptosis was assessed by TUNEL staining after LPS. Finally, the expression of autophagy-associated proteins and inflammasome-associated proteins in lung tissue after LPS intervention was analyzed by western blot. We found that wild-type control, FUNDC1 knockout control, lipopolysaccharide-induced wild-type, and FUNDC1 knockout mouse models were used to investigate whether FUNDC1-mediated autophagy is involved in lung injury and its possible molecular mechanisms. Compared with the normal control group, lung tissue FUNDC1 and LC3 II increased and p62/SQSTM1 decreased after LPS intervention, and increased ROS levels led to a decrease in corresponding antioxidant enzymes along with an increased inflammatory response and apoptosis. Levels of autophagy in lipopolysaccharide-induced mice deficient in FUNDC1 were significantly decreased, but the expression of ROS and inflammatory factors in lung tissue was more severe than in lipopolysaccharide-induced wild-type mice, and the survival rate was significantly decreased. Western blot analysis showed that autophagy was significantly inhibited in the FUNDC1 KO+LPS group, and there was a significant increase in NLRP3, caspase-1, IL-1β, and ASC compared with the lipopolysaccharide-induced wild-type group. In summary, lipopolysaccharide-induced wild-type mice exhibit ROS-dependent activation of autophagy, and knocking out FUNDC1 promotes inflammasome activation and exacerbates lung injury.
急性呼吸窘迫综合征(ARDS)的发病率和死亡率很高,但其发病机制尚不清楚。自噬在ARDS的发展中起重要作用。线粒体外膜蛋白FUNDC1参与缺氧介导的线粒体自噬,这可能有助于ARDS的发展。本研究在脂多糖诱导的小鼠模型中探讨FUNDC1是否通过抑制ROS-NLRP3信号通路调节自噬以避免肺部细胞凋亡。本研究构建了FUNDC1基因敲除小鼠,并建立了脂多糖诱导的小鼠模型。通过对肺组织病理切片进行HE染色、测量肺组织湿/干重、检测BALF中的髓过氧化物酶浓度/中性粒细胞计数以及小鼠的存活时间来确定建模效果。采用ELISA法评估BALF和血浆中LPS刺激后细胞因子(TNF-α、IL-1β、IL-6和IL-10)的释放情况。通过生化分析检测肺组织中LPS刺激后的氧化应激(丙二醛、超氧化物歧化酶、过氧化氢酶、谷胱甘肽过氧化物酶)效应。通过iNOS染色验证氧化应激损伤,LPS刺激后通过TUNEL染色评估细胞凋亡。最后,通过蛋白质免疫印迹法分析LPS干预后肺组织中自噬相关蛋白和炎性小体相关蛋白的表达。我们发现使用野生型对照、FUNDC1基因敲除对照、脂多糖诱导的野生型和FUNDC1基因敲除小鼠模型来研究FUNDC1介导的自噬是否参与肺损伤及其可能的分子机制。与正常对照组相比,LPS干预后肺组织中FUNDC1和LC3 II增加,p62/SQSTM下降,ROS水平升高导致相应抗氧化酶减少,同时炎症反应和细胞凋亡增加。FUNDC1基因敲除的脂多糖诱导小鼠的自噬水平显著降低,但肺组织中ROS和炎性因子的表达比脂多糖诱导的野生型小鼠更严重,存活率显著降低。蛋白质免疫印迹分析显示,FUNDC1基因敲除+LPS组自噬被显著抑制,与脂多糖诱导的野生型组相比,NLRP3、caspase-1、IL-1β和ASC显著增加。总之,脂多糖诱导的野生型小鼠表现出ROS依赖性的自噬激活,敲除FUNDC1会促进炎性小体激活并加重肺损伤。
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