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镍化合物体外诱导人血淋巴细胞染色体和核染色质中的DNA单链断裂:氧化应激和细胞内钙的作用

Nickel compound-induced DNA single-strand breaks in chromosomal and nuclear chromatin in human blood lymphocytes in vitro: role of oxidative stress and intracellular calcium.

作者信息

M'Bemba-Meka Prosper, Lemieux Nicole, Chakrabarti Saroj K

机构信息

Human Toxicology Research Group (TOXHUM), Department of Environmental and Occupational Health, Faculty of Medicine, Université de Montréal, P.O. Box 6128, Main Station, Montréal, Que., Canada H3C 3J7.

出版信息

Mutat Res. 2005 Oct 3;586(2):124-37. doi: 10.1016/j.mrgentox.2005.06.001.

Abstract

The effects of nickel sulfate, and soluble forms of nickel carbonate hydroxide (NiCH), nickel subsulfide, and nickel oxide on delayed induction of DNA single-strand breaks (DNA SSBs) in chromosomal and nuclear chromatin of human blood lymphocytes in culture were studied. After 46 h of initial culture in supplemented RPMI-1640 media at 37 degrees C, human whole blood lymphocytes in culture were exposed to low concentrations (0-15 microM) of different nickel (Ni) compounds for 2 h, whereas only RPMI-1640 medium served as control. Immediately after 2 h of such exposure, both control and Ni-treated cells were washed with the same medium and incubated further in fresh complete RPMI-1640 culture medium for another 24h. After a total 70 h of incubation, cells were then arrested at metaphase. Two hours later, the induction of DNA SSBs involving both metaphase chromosomal and interphase nuclear chromatin was measured using the method of electron microscopy in situ end-labeling. The metaphase chromosomal chromatin showed significantly higher DNA SSBs (as measured by an increase in immunogold particles per microm2 chromatin) due to 15 microM NiCH and NiO when compared to the corresponding control value. Both NiCH and nickel oxide produced significantly higher induction of DNA SSBs than those of nickel subsulfide and nickel sulfate in chromosomal chromatin. The DNA SSBs in chromosomal chromatin were found to be significantly higher than those in nuclear chromatin due to different Ni compounds. Overall, the genotoxic potency seems to be decreased as follows: NiCH>nickel oxide>or=nickel subsulfide>nickel sulfate. Pretreatment of human blood lymphocytes with either catalase (a H2O2 scavenger), or superoxide dismutase (a scavenger of O2- radical) or dimethylthiourea (a hydroxyl radical scavenger), or N-acetylcysteine (GSH precursor) significantly reduced DNA SSBs in both chromosomal and nuclear chromatin induced by NiCH, suggesting the involvement of different types of oxidative stress in such genotoxicity. Deferoxamine (a highly specific iron chelator) pretreatment prevented NiCH-induced DNA SSBs in both chromosomal and nuclear chromatin suggesting a role of iron-mediated oxidative stress generating hydroxyl radical in such genotoxicity. Simultaneous treatment with either verapamil (an inhibitor of Ca 2+ through plasma membranes), or dantrolene (an inhibitor of mobilization of [Ca2+]i from endoplasmic reticulum), or BAPTA (a Ca2+ chelator) significantly reduced Ni compound-induced DNA SSBs in both chromosomal and nuclear chromatin, suggesting that Ni compound-induced destabilization of calcium homeostasis may also involved in the induction of such DNA SSBs.

摘要

研究了硫酸镍、氢氧化镍碳酸酯(NiCH)的可溶形式、硫化亚镍和氧化镍对培养的人血淋巴细胞染色体和核染色质中DNA单链断裂(DNA SSB)延迟诱导的影响。在补充了RPMI - 1640培养基的条件下于37℃初始培养46小时后,将培养的人全血淋巴细胞暴露于低浓度(0 - 15 microM)的不同镍(Ni)化合物中2小时,而仅RPMI - 1640培养基作为对照。在这种暴露2小时后,立即用相同培养基洗涤对照细胞和经镍处理的细胞,并在新鲜的完全RPMI - 1640培养基中进一步孵育24小时。总共孵育70小时后,将细胞阻滞在中期。两小时后,使用原位末端标记电子显微镜方法测量涉及中期染色体和间期核染色质的DNA SSB的诱导情况。与相应的对照值相比,中期染色体染色质显示由于15 microM的NiCH和NiO导致DNA SSB显著更高(通过每平方微米染色质中免疫金颗粒的增加来衡量)。在染色体染色质中,NiCH和氧化镍产生的DNA SSB诱导均显著高于硫化亚镍和硫酸镍。由于不同的镍化合物,发现染色体染色质中的DNA SSB显著高于核染色质中的DNA SSB。总体而言,遗传毒性效力似乎按以下顺序降低:NiCH>氧化镍>或=硫化亚镍>硫酸镍。用过氧化氢酶(一种H2O2清除剂)、超氧化物歧化酶(一种O2-自由基清除剂)、二甲基硫脲(一种羟基自由基清除剂)或N - 乙酰半胱氨酸(谷胱甘肽前体)对人血淋巴细胞进行预处理,可显著降低NiCH诱导的染色体和核染色质中的DNA SSB,表明不同类型的氧化应激参与了这种遗传毒性。去铁胺(一种高度特异性的铁螯合剂)预处理可预防NiCH诱导的染色体和核染色质中的DNA SSB,表明铁介导的产生羟基自由基的氧化应激在这种遗传毒性中起作用。同时用维拉帕米(一种通过质膜的Ca2+抑制剂)、丹曲林(一种从内质网动员[Ca2+]i的抑制剂)或BAPTA(一种Ca2+螯合剂)处理,可显著降低镍化合物诱导的染色体和核染色质中的DNA SSB,表明镍化合物诱导的钙稳态失衡也可能参与了这种DNA SSB的诱导。

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