天然除虫菊素诱导人肝细胞DNA氧化损伤研究  

作　　者：杨韵 应梦超 孙静秋[1] 沙毅杰 洪新宇[1] 肖萍[1] 陶功华[1] YANG Yun;YING Mengchao;SUN Jingqiu;SHA Yijie;HONG Xinyu;XIAO Ping;TAO Gonghua(In vitro Toxicological Laboratory,Shanghai/State Environmental Protection Key Laboratory of the Assessment of Effects of Emerging Pollutants on Environmental and Human Health/NMPA Key Laboratory for Monitoring and Evaluation of Cosmetics,Shanghai Municipal Center for Disease Control and Prevention,Shanghai 200336,China)

机构地区：[1]上海市疾病预防控制中心体外毒理检测与评价室/国家环境保护新型污染物环境健康影响评价重点实验室/国家药品监督管理局化妆品监测评价重点实验室,上海200336

出　　处：《环境与职业医学》2024年第6期681-686,共6页Journal of Environmental and Occupational Medicine

基　　金：上海市青年科技英才扬帆计划项目(21YF1439100);上海市公共卫生体系建设三年行动计划重点学科建设项目(GWVI-11.1-41);国家环境保护重点实验室新兴污染物环境健康影响评价专项基金项目(SEPKL-EHIAEC-202204);上海市卫生健康委员会卫生行业临床研究专项面上项目(202140489)。

摘　　要：[背景]天然除虫菊素被广泛应用于环境和家庭卫生领域。研究显示,其具有潜在的肝脏毒性,但具体机制尚不明确。[目的]探讨天然除虫菊素对人肝细胞DNA损伤的影响。[方法]本研究以人肝细胞QSG7701为体外测试模型,以未处理细胞为对照组,以经系列质量浓度(后称浓度)(5、10、20和40μg·mL^(−1))天然除虫菊素暴露6 h或24 h后作为处理组。分别采用荧光探针法经荧光显微镜检测细胞活性氧(ROS)的荧光强度;采用比色法经酶标仪检测细胞内硫代巴比妥酸反应物质(TBARS)的水平;采用彗星电泳试验镜下观察DNA断片迁移以检测DNA损伤程度;采用免疫荧光试验通过激光共聚焦对细胞磷酸化H2AX(γH2AX)及8-氧鸟嘌呤(8-oxoG)水平等指标进行检测。[结果]随着天然除虫菊素浓度的升高,ROS荧光强度呈剂量依赖性升高,与对照组相比,10μg·mL^(−1)及以上浓度组差异均有统计学意义(P<0.01),其中20μg·mL^(−1)和40μg·mL^(−1)处理组ROS水平是对照组的2.17和3.05倍;TBARS水平随着天然除虫菊素浓度升高而升高(P<0.01),20μg·mL^(−1)和40μg·mL^(−1)天然除虫菊素处理组的TBARS水平是对照组2.46和3.01倍;彗星试验结果显示,各浓度组细胞DNA呈现不同程度的拖尾,随着天然除虫菊素暴露浓度的增高,尾部DNA含量(TDNA%)、尾长(TL)、尾矩(TM)和Olive尾矩(OTM)等指标呈剂量依赖性增高,与对照组相比,20μg·mL^(−1)及以上浓度组差异均有统计学意义(P<0.01),其中40μg·mL^(−1)浓度组TDNA%、TL、TM及OTM指标分别为(46.92±3.52)%、(64.67±4.16)μm、30.96±2.94和22.64±3.89。细胞免疫荧光结果显示天然除虫菊素可诱导γH2AX和8-oxoG的形成,且荧光强度呈剂量依赖性增高,与对照组相比,在10μg·mL^(−1)及以上浓度组相对荧光强度的增高均有统计学意义(P<0.01)。[结论]天然除虫菊素可诱导人肝细胞DNA损伤,且ROS介导的氧化应激可能在其诱导的肝细胞遗传�[Background]Natural pyrethrins have long been widely used in the fields of environmental and household hygiene.Studies have reported that natural pyrethrins have potential liver toxicity,but their specific mechanisms are still unclear yet.[Objective]To explore the effect of natural pyrethrins on DNA damage in human liver cells.[Methods]This study used human liver cell QSG7701 as an in vitro testing model.After exposure to DMSO and a series of concentrations of natural pyrethrins(5,10,20,and 40μg·mL^(−1))for 6 and 24 h,reactive oxygen species(ROS)was detected by fluorescence microscopy using a fluorescence probe,thiobarbituric acid reactive substance(TBARS)by colorimetric method using a microplate reader,DNA damage by comet assay through observing DNA fragment migration under microscope,and phospho H2AX(γH2AX)and 8-oxoguanine(8-oxoG)by immunofluorescence assay using a laser confocal microscope.[Results]As the exposure concentration of natural pyrethrins increased,the fluorescence intensity of ROS significantly increased in a concentration-dependent manner.The differences in ROS between the 10μg·mL^(−1) and above groups and the control group were statistically significant(P<0.01),and the ROS levels in the 20μg·mL^(−1) and 40μg·mL^(−1) treatment groups were 2.17 and 3.05 times higher than that in the control group respectively.The TBARS level increased in a concentration-dependent manner in natural pyrethrins treated cells(P<0.01),and the levels in the 20μg·mL^(−1) and 40μg·mL^(−1) treatment groups were 2.46 and 3.01 times higher than that in the control group respectively.The results of comet assay showed trailing formation of cellular DNA in each dose group;as the exposure concentration of natural pyrethrins increased,indicators such as tail DNA content(TDNA%),tail length(TL),tail moment(TM),and Olive tail moment(OTM)increased in a concentration-dependent manner.Compared with the control group,the differences in the indicators between the 20μg·mL^(−1) and above groups and the control g

关 键 词：天然除虫菊素 人肝细胞 活性氧 氧化应激 DNA损伤 遗传毒性 

分 类 号：R114[医药卫生—卫生毒理学]