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汪海涛, 林洁, 杨波, 朱宏丽, 李素霞, 范辉, 郭搏, 冉海红, 翟冰, 刘洋, 李宝玲, 张文英, 李建华, 杜鑫. 过氧化氢诱导人巨核细胞系Dam i氧化应激模型的建立及评价[J]. 解放军医学院学报, 2014, 35(4): 349-352,356. DOI: 10.3969/j.issn.2095-5227.2014.04.015
引用本文: 汪海涛, 林洁, 杨波, 朱宏丽, 李素霞, 范辉, 郭搏, 冉海红, 翟冰, 刘洋, 李宝玲, 张文英, 李建华, 杜鑫. 过氧化氢诱导人巨核细胞系Dam i氧化应激模型的建立及评价[J]. 解放军医学院学报, 2014, 35(4): 349-352,356. DOI: 10.3969/j.issn.2095-5227.2014.04.015
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WANG Hai-tao, LIN Jie, YANG Bo, ZHU Hong-li, LI Su-xia, FAN Hui, GUO Bo, RAN Hai-hong, ZHAI Bing, LIU Yang, LI Bao-ling, ZHANG Wen-ying, LI Jian-hua, DU Xin. Hydrogen peroxide-induced oxidative stress model of human megakaryocytic Dami cells and its assessment[J]. ACADEMIC JOURNAL OF CHINESE PLA MEDICAL SCHOOL, 2014, 35(4): 349-352,356. DOI: 10.3969/j.issn.2095-5227.2014.04.015
Citation: WANG Hai-tao, LIN Jie, YANG Bo, ZHU Hong-li, LI Su-xia, FAN Hui, GUO Bo, RAN Hai-hong, ZHAI Bing, LIU Yang, LI Bao-ling, ZHANG Wen-ying, LI Jian-hua, DU Xin. Hydrogen peroxide-induced oxidative stress model of human megakaryocytic Dami cells and its assessment[J]. ACADEMIC JOURNAL OF CHINESE PLA MEDICAL SCHOOL, 2014, 35(4): 349-352,356. DOI: 10.3969/j.issn.2095-5227.2014.04.015
shu

过氧化氢诱导人巨核细胞系Dam i氧化应激模型的建立及评价

Hydrogen peroxide-induced oxidative stress model of human megakaryocytic Dami cells and its assessment

    摘要
  • 摘要: 目的 探讨过氧化氢(H2O2)诱导Dami细胞氧化应激模型的条件,建立并评价模型。 方法 不同浓度过氧化氢处理Dami细胞后,Giemsa染色,显微镜观察细胞形态学的变化;CCK-8试剂盒检测细胞增殖活性,绘制生长曲线,计算半数抑制浓度(IC50);加载DCFH-DA探针后流式细胞仪检测细胞内活性氧自由基水平;Western blot检测核因子NF-E2相关因子(Nrf2)、醌氧化还原酶(NQO1)、血红素加氧酶(HO-1)、γ-谷氨酰半胱氨酸合成酶催化亚单位(GCLC)表达量。 结果 随着H2O2浓度升高,Dami细胞核皱缩趋于明显,存活率下降,IC50为(0.9132±0.144) mmol/L;0.1 mmol/L、1 mmol/L、10 mmol/L H2O2处理Dami细胞2 h,细胞氧化应激阳性率分别为12.11%、20.91%、52.53%;H2O2处理Dami细胞24 h后,抗氧化蛋白Nrf2、GCLC水平升高,未检测到HO-1和NQO1的表达。 结论 1 mmol/L H2O2是建立Dami细胞氧化应激模型的合适浓度。Dami细胞抗氧化应激反应与Nrf2/ARE通路有关。

     

    Abstract: Objective To establish and assess the H2O2-induced oxidative stress model of Dami cells. Methods Morphology of Giemsa-stained Dami cells was observed under microscope after they were treated with H2O2 at different concentrations. Proliferation of Dami cells was assayed with CCK-8 kit. Growth curve of Dami cells was plotted and 50% inhibiting concentration (IC50) of H2O2 was calculated. ROS levels in Dami cells were measured by Flow cytometry after DCFH-DA probe was loaded. Nrf2, NQO1, HO-1, and γ-GCLC expressions were detected by Western blot. Results The shrinkage of Dami cells increased and their survival rate decreased with the increasing H2O2 concentration. The IC50 of H2O2 was 0.9132 ± 0.144 mmol/L 2 h after the Dami cells were treated at the concentration of 0.1, 1, and 10 mmol/L, respectively. The positive oxidative stress rate of Dami cells was 12.11%, 20.91%, and 52.53%, respectively. The expression levels of Nrf2 and γ-GCLC were higher 24 h after the Dami cells were treated with H2O2. However, no expression of HO-1 and NQO1 was detected. Conclusion Oxidative stress model of Dami cells can be established with H2O2 at the concentration of 1 mmol/L and anti-oxidative stress of Dami cells is associated with the Nrf2/ARE pathway.

     

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