丁基苯酞对过氧化氢诱导下视网膜Mǖller细胞凋亡的影响  被引量：8

作　　者：邢小丽 黄亮瑜 苏睿虹 刘勋 赵今稚 高美子 张晓敏[1] 李筱荣[1] 东莉洁[1] Xing Xiaoli;Huang Liangyu;Su Ruihong;Liu Xun;Zhao Jinzhi;Gao Meizi;Zhang Xiaomin;Li Xiaorong;Dong Lijie(Tianjin Medical University Eye Hospital,Tianjin Medical University Eye Institute,College of Optometry and Ophthalmology,Tianjin 300384,China)

机构地区：[1]天津医科大学眼科医院天津医科大学眼科研究所天津医科大学眼视光学院,300384

出　　处：《中华眼底病杂志》2018年第5期481-486,共6页Chinese Journal of Ocular Fundus Diseases

基　　金：国家自然科学基金（81570872）;天津市卫计委青年医学新锐人才项目;天津市应用基础与前沿技术研究计划（15JCYBJC24900）;天津医科大学自然科学基金（2016KYZM16）;天津医科大学眼科研究所科研临床基金（15YKYJS001）;天津医科大学校级基金（2006KY27）

摘　　要：目的观察丁基苯酞（NBP）对过氧化氢（H2O2）诱导下视网膜Müller细胞凋亡的保护作用。方法体外培养的人视网膜Müller细胞分为正常对照组、模型组（H2O2组）、实验组（H2O2＋NBP组）。H2O2组、H2O2＋NBP组细胞培养液中加入200 μmol/L H2O2刺激2 h后，H2O2组更换为完全培养基，H2O2＋NBP组更换为含1 μmol/L NBP的完全培养基。正常对照组为常规培养细胞。苏木精-伊红（HE）染色观察各组细胞形态改变；噻唑蓝（MTT）比色法检测NBP作用24、48 h后各组细胞活性；Hoechst33258染色观察各组细胞凋亡情况；LIVE/DEAD细胞活性/细胞毒性试剂盒检测各组细胞生存力；二氯荧光素二乙酸酯（DCFH-DA）＋内质网（ER）红色荧光探针（ER-Tracker Red）双染色观察各组细胞ER中活性氧（ROS）的表达水平。单因素方差分析联合Dunnett统计学方法进行数据分析。结果HE染色结果显示，H2O2＋NBP组细胞数量较H2O2组增加。MTT比色法检测结果发现，NBP作用24、48 h后，正常对照组与H2O2组、H2O2组与H2O2＋NBP组细胞生存力比较，差异均有统计学意义（t=28.96、3.658、47.58、20.33，P＜0.001、0.022）。Hoechst33258结果显示，H2O2＋NBP组细胞少数细胞核边集呈新月状且细胞核碎裂减少，其余细胞蓝色荧光均匀。LIVE/DEAD细胞活性/细胞毒性试剂盒检测结果显示，H2O2组中呈红色荧光的死亡细胞明显增多，呈绿色荧光的活细胞数量显著减少；H2O2＋NBP组呈绿色荧光的活细胞数量增多，呈红色荧光的死亡细胞减少。DCFH-DA＋ER-Tracker Red双染色结果显示，H2O2组细胞中绿色荧光强度明显增强；H2O2＋NBP组细胞中绿色荧光强度较H2O2组明显降低。结论NBP通过抑制ROS的产生缓解H2O2诱导的人视网膜Müller细胞凋亡。ObjectiveTo observe the protective effect of dl-3-n-Butylphthalide （NBP） on apoptosis of retinal Müller cells induced by hydrogen peroxide （H2O2）.MethodsHuman retinal Müller cells cultured in vitro were divided into normal control group, model group （H2O2 group） and experimental group （H2O2＋NBP group）. The cells in the H2O2 group and H2O2＋NBP group were cultured with 200 μmol/L H2O2 for 2 h. Then the culture solution of the H2O2 group replace with complete medium and the H2O2＋NBP group replace with complete medium containing 1 μmol/L NBP. The normal control group was a conventional cultured cells. Müller cells were identified by immunofluorescence staining. Hematoxylin-eosin （HE） staining was used to observe the apoptosis morphological changes. MTT assay was used to detect the activity of of retinal Müller cells after after 24 h and 48 h of NBP intervention. Hoechst33258 staining was used to observe the apoptosis. LIVE/DEAD cell activity/cytotoxicity kit was used to detect cell viability. Dichlorofluorescein diacetate （DCFH-DA） ＋ endoplasmic reticulum （ER） red fluorescent probe （ER-Tracker Red） double staining was used to observe the expression level of reactive oxygen species （ROS） in ER of cells. One-way ANOVA combined with Dunnett statistical method were used for data analysis.ResultsHE staining showed that the number of cells in H2O2＋NBP group was higher than that in H2O2 group. MTT assay showed that after 24 h and 48 h of NBP intervention, the differences in cell viability between the normal control group and the H2O2 group, the H2O2 group and the H2O2＋NBP group were statistically significant （t=28.96, 3.658, 47.58, 20.33; P〈0.001, 0.022）. The results of Hoechst33258 showed that the nuclear nucleus of a few cells in the H2O2＋NBP group was crescent-shaped and the nuclear fragmentation was reduced, and the blue fluorescence of the remaining cells was uniform. The LIVE/DEAD cell activity/cytotoxicity kit showed that the number of dead cells with re

关 键 词：丁基苯酞 氧化应激 细胞凋亡 过氧化氢 Mǖller细胞 

分 类 号：R774[医药卫生—眼科]