摘要
二氢青蒿素(dihydroartemisinin,D H A)是青蒿素的一种衍生物,在多种肿瘤中表现出明显的抗肿瘤活性,但其具体机制不详。本文探讨了D H A对肝癌细胞的毒性作用机制。利用C C K-8试剂检测D H A对肝癌细胞株活力的影响,通过荧光探针染色及流式细胞术分析细胞内R 0 S及脂质过氧化物水平的变化;通过谷胱甘肽测定试剂盒检测细胞内还原型谷胱甘肽含量的变化,并通过免疫印迹分析D H A作用下细胞内铁死亡通路蛋白质中G P X 4的变化。结果发现,D H A能显著抑制SMMC-7721及H uh-7细胞活力,其半数抑制浓度分别为23.74 p m o l/L及26.92 jjumol/L。在35 pm ol/L D H A处理下,SMMC-7721及H uh-7细胞内R 0 S分别升高2.6倍和2.1倍,月旨质过氧化物升高2.3倍和1.7倍。D H A可诱导细胞内G SH含量下降,并能下调铁死亡相关蛋白质G P X 4蛋白水平。通过利用小分子抑制剂进行功能恢复实验发现,R 0 S抑制剂、铁螯合剂及铁死亡抑制剂都可不同程度恢复D H A引起的细胞活力下降。进一步检测发现,铁死亡抑制剂可抑制D H A诱导的脂质过氧化,并恢复G SH含量及G P X 4蛋白水平。结果表明,在肝癌细胞中,D H A可通过诱导细胞发生铁死亡抑制肝癌细胞生长。
Dihydroartemisinin(D H A),a derivative of artemisinin,has been identified as critical and promising agent for targeting human cancers,including hepatocellular carcinoma(H C C).However,the anticancer role of DHA in HCC and its underlying mechanism are still illusive.The aim of this study was to explore the toxic mechanism of DHA to hepatocellular carcinoma cells.CCK-8 reagent was used to detect the effect of DHA on human hepatocellular carcinoma cell viability.The changes of intracellular ROS and lipid peroxide levels were analyzed by fluorescence probe staining and flow cytometry.The glutathione assay kit was used to determine cellular reduced glutathione(GSH)content and the protein level of GPX4,a marker protein in ferroptosis,was tested by Western blot.The results showed that DHA can significantly inhibit SMMC-7721 and Huh-7 cell viabilities,with the half-inhibitory concentrations of 23.74μxmol/L and 26.92 jxmol/L,respectively.Under the treatment of 35μmol/L DHA,the ROS in SMMC-7721 and Huh-7 cells increased by 2.6-fold and 2.1-fold,respectively,and lipid peroxides increased by 2.3-fold and 1.7-fold.DHA induced a decrease of GSH amount and GPX4 protein level.Further rescue experiments exhibited that different small molecule inhibitors,like ROS inhibitors,iron chelating agents or ferroptosis inhibitors,could restore the decreased cell viability caused by DHA to different degrees.More tests demonstrated that ferroptosis inhibitor diminished the lipid peroxidation induced by DHA and reversed the GSH content and GPX4 protein levels.These results suggest that DHA inhibits hepatocellular carcinoma cell growth by inducing ferroptosis.
作者
李艳纯
周怡
王鑫
王旭
陈素峰
王莹
杜璟
LI Yan-Chun;ZHOU Yin;WANG Xing;WANG Xu;CHEN Su-Feng;WANG Ying;DU Jing(Second Clinical Medical School of Zhejiang Chinese Medical University,Hangzhou 310053,China;Clinical Research Institute,Zhejiang Provincial People’s Hospital,People's Hospital of Hangzhou Medical College,Hangzhou 310014,China;Department o f Laboratory Medicine,Zhejiang Provincial People's Hospital,People's Hospital of Hangzhou Medical College,Hangzhou 310014,China)
出处
《中国生物化学与分子生物学报》
CAS
CSCD
北大核心
2019年第12期1361-1366,共6页
Chinese Journal of Biochemistry and Molecular Biology
基金
浙江省公益技术应用研究计划(No.LGF19H080006)
浙江省医药卫生科技计划(No.2019RC014,2019RC115,2017KY006,2015KYB024)
浙江省人民医院优秀青年启动基金(No.ZRY2016B007,ZRY2016A003)
浙江省大学生科技创新活动计划(No.2019R410053)资助~~
关键词
二氢青蒿素
肝癌
铁死亡
脂质过氧化物
dihydroartemisinin(DHA)
hepatocellular carcinoma(HCC)
ferroptosis
lipid peroxide