机构地区:[1]贵州医科大学卫生毒理学教研室、环境污染与疾病监控省部共建教育部重点实验室,贵州550025
出 处:《中华地方病学杂志》2016年第6期412-416,共5页Chinese Journal of Endemiology
基 金:国家自然科学基金(81360411、81430077)志谢在生物样本采集及实验实施中给予帮助的岑延利、李昌哲、谢婷婷、王庆陵、邹忠兰
摘 要:目的观察贵州省燃煤污染型砷中毒病区砷暴露者外周血细胞组蛋白H4第20位赖氨酸(H4K20)甲基化修饰水平及其与血细胞DNA损伤的关系,为揭示砷抑制DNA损伤修复机制研究提供依据。方法以贵州省兴仁县燃煤型砷中毒病区交乐村为调查点,通过健康体检,选择115例砷暴露者为砷暴露组;同时选择相邻的非病区上坝田村53例居民作为对照组。采集观察对象发样、外周血,提取血细胞组蛋白;微波消解-电感耦合等离子质谱(ICP—MS)法测定发样中砷元素的含量;酶联免疫吸附实验(ELISA)检测外周血细胞组蛋白H4K20一、二、三甲基化(H4K20me1、me2、me3)修饰水平;单细胞凝胶电泳(SCGE)法检测DNA损伤。结果发砷含量测定结果:与对照组[中位数(M,四分位数):0.12(0.08~0.18)μg/g]比较,砷暴露组发砷[M(四分位数):0.30(0.19-0.46)μg/g]含量明显升高(F=11.968,P〈0.05)。H4K20甲基化修饰水平检测结果:与对照组(0.44±0.14、0.99±0.41、1.06±0.33)比较,砷暴露组H4K20mel修饰水平(0.60±0.29)升高(F=2.513,P〈0.05)、H4K20me2修饰水平(0.75±0.26)降低(F=4.707,P〈0.05)、H4K20me3修饰水平(1.20±0.62)变化不明显(F=0.582,P〉0.05)。DNA损伤检测结果:与对照组[M:2.12、1.16]比较,砷暴露组尾部DNA百分含量(TailDNA%,M:10.75)、Olive尾矩(Olivetailmoment,M:11.69)均明显升高(F=9.307、9.457,P均〈0.05)。相关性分析:观察对象H4K20me1修饰水平与发砷含量呈正相关r=0.214,P〈0.05),H4K20me2修饰水平与其呈负相关关系(r=-0.224,P〈0.05);H4K20me1修饰水平与DNA损伤水平(TailDNA%、Olivetailmoment)均呈正相关关系(r=0.383、0.380,P均〈0.05),H4K20me2修饰水平与其均呈负相关关系(r=-0.290、-0.298,P均〈0.Objective To detect the global level of histone 4 lysine 20 (H4K20) methylation and its relation with DNA damage-repair in peripheral blood cell of arsenic-exposed residents in the coal-contaminated arsenism areas in Guizhou, in order to provide a basis to deepen the interpretation of the role of arsenic in inhibiting DNA damage-repair. Methods Jiaole village in coal-burning-borne arsenism areas in Xingren County of Guizhou was selected as the survey point, and 115 cases of arsenic-exposed residents were selected as the arsenic exposed group on the basis of physical examination. Moreover, 53 residents from one village of non-epidemic area neighboring the diseased area were selected as controls. Hair and peripheral blood samples of these subjects were collected, and the histone protein was extracted from the lymphocytes separated from blood samples. The hair samples were digested with microwave digestion instrument, and the hair arsenic content was tested via the inductively coupled plasma-mass spectrometry (ICP-MS) method; the level of H4K20 1, 2, 3 methylation (H4K20me2, me2, me3) in peripheral blood cell was tested by enzyme-linked immunosorbent assay (ELISA); DNA damage of peripheral blood cell was measured by single cell gel electrophoresis (SCGE). Results The testing results of hair arsenic contents showed that the arsenic levels of hair in arsenic exposed group [0.30 (0.19 - 0.46) μg/g] were significantly higher than those of control group [0.12 (0.08 - 0.18) μg/g, F = 11.968, P 〈 0.05]. Compared with the eontrol (0.44 ± 0.14, 0.99 ± 0.41, 1.06 ± 0.33), the level of H4K20mel (0.60 ± 0.29) in arsenic exposed group was higher (F = 2.513, P 〈 0.05), H4K20me2 (0.75± 0.26) was lower (F = 4.707, P 〈 0.05), and H4K20me3 (1.20± 0.62) was of no significant difference (F = 0.582, P 〉 0.05). The detecting results of DNA damage of the lymphocytes separated from peripheral blood showed a statistically significant increase (F = 9.307, 9.457, all P
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