环境化学污染物暴露相关基因甲基化焦磷酸测序方法的构建和应用

doi:10.3969/j.issn.1004-616x.2017.02.001

癌变·畸变·突变 ›› 2017, Vol. 29 ›› Issue (2): 81-86.doi: 10.3969/j.issn.1004-616x.2017.02.001

• 论著 • 下一篇

环境化学污染物暴露相关基因甲基化焦磷酸测序方法的构建和应用

张海燕, 黎青叶, 陈燊, 陈雯, 何志妮

中山大学公共卫生学院预防医学系, 广东广州 510080

收稿日期:2016-12-06 修回日期:2017-02-26 出版日期:2017-03-31 发布日期:2017-03-31
通讯作者: 何志妮,E-mail:383179088@qq.com E-mail:383179088@qq.com
作者简介:张海燕,E-mail:752665535@qq.com。
基金资助:
国家自然科学基金重大研究计划项目（91543208）

Construction of an environmental pollution-responsive gene-specific pyrosequencing assay

ZHANG Haiyan, LI Qingye, CHEN Shen, CHEN Wen, HE Zhini

Faculty of Preventive Medicine, School of Public Health, Sun Yat-sen University, Guangzhou 510080, Guangdong, China

Received:2016-12-06 Revised:2017-02-26 Online:2017-03-31 Published:2017-03-31

摘要/Abstract

摘要：

目的：构建适用于环境化学污染物暴露相关基因甲基化的焦磷酸测序方法，应用于检测多环芳烃暴露的焦炉工人外周血细胞DNA的基因甲基化修饰。方法：采用亚硫酸氢盐修饰后测序检测多环芳烃职业暴露工人外周血中RAS相关结构域家族基因1A（RASSF1A）的甲基化水平，选择对暴露因素响应明显，即在两组人群中存在显著统计学差异的甲基化位点较集中的片段作为甲基化敏感区域。针对该区域构建焦磷酸测序方法，并在焦炉工人中进行验证。结果：所构建的焦磷酸测序方法具有更快速、简便、准确及经济的特点，能有效区分多环芳烃职业暴露工人与对照工人，其中，焦炉暴露工人RASSF1A甲基化修饰水平升高了87.15%（暴露组为9.32%±3.82%，对照工人为4.98%±2.28%，P < 0.01）。结论：基于外源性化学物暴露人群的亚硫酸氢盐修饰后测序结果选取焦磷酸测序片段具有良好的化学物特异性和准确度，可用于职业暴露人群大样本DNA甲基化检测。

关键词: 焦磷酸测序, 多环芳烃类物质, 职业暴露, DNA甲基化, 生物学标志

Abstract:

OBJECTIVE: To establish a pollutant-responsive gene-specific pyrosequencing assay for quantitative measurement of DNA methylation in peripheral blood lymphocytes of coke-oven workers. METHODS: We firstly analyzed DNA methylation levels of RAS-associated domain family 1 (RASSF1A) in 69 coke-oven workers and 46 controls using bisulfate sequencing method. The hyper-methylated hotspots in the exposure group were recognized as the target region for design of specific primers of pyrosequencing. As a pilot study,we examined the methylation status of RASSF1A in 11 paired coke-oven workers and controls. RESULTS: Pyrosequencing was the optimized assay for DNA methylation detection. Compared to BSP assay,pyrosequencing exhibited advantages in efficiency,simplicity,accuracy and economical performances. We were able to distinguish occupational exposed workers from controls effectively using this method. The methylation level of RASSF1A in coke-oven workers was increased by 87.15% compared to that in the controls (9.32%±3.82% and 4.98%±2.28%,respectively,P < 0.01). CONCLUSION: Compared to the BSP assay, gene-specific pyrosequencing method exhibited strength in specificity and accuracy of methylation detection of environmental pollutant-responsive gene in PAHs-exposed workers.

Key words: pyrosequencing, PAHs, occupational exposure, DNA methylation, biomarkers

中图分类号:

R114

张海燕, 黎青叶, 陈燊, 陈雯, 何志妮. 环境化学污染物暴露相关基因甲基化焦磷酸测序方法的构建和应用[J]. 癌变·畸变·突变, 2017, 29(2): 81-86.

ZHANG Haiyan, LI Qingye, CHEN Shen, CHEN Wen, HE Zhini. Construction of an environmental pollution-responsive gene-specific pyrosequencing assay[J]. Carcinogenesis, Teratogenesis & Mutagenesis, 2017, 29(2): 81-86.

参考文献

[1] VANIUSHIN B F. DNA methylation and its biological significance [J]. Usp Sovrem Biol,1968,65(2):163-185.

[2] FEINBERG A P,TYCKO B. The history of cancer epigenetics [J]. Nat Rev Cancer,2004,4(2):143-153.

[3] GRONBAEK K,TREPPENDAHL M,ASMAR F,et al. Epigenetic changes in cancer as potential targets for prophylaxis and maintenance therapy[J]. Basic Clin Pharmacol Toxicol,2008,103(5):389-396.

[4] HUBERS A J,HEIDEMAN D A,BURGERS S A,et al. DNA hypermethylation analysis in sputum for the diagnosis of lung cancer:training validation set approach[J]. Br J Cancer,2015,112(6):1105-1113.

[5] FU D Y,REN C L,TAN H S,et al. Sox17 promoter methylation in plasma DNA is associated with poor survival and can be used as a prognostic factor in breast cancer[J]. Medicine,2015,94(11):e637.

[6] PASTUSZAK-LEWANDOSKA D,KORDIAK J,ANTCZAK A,et al. Expression level and methylation status of three tumor suppressor genes,DLEC1,ITGA9 and MLH1,in non-small cell lung cancer[J]. Med Oncol,2016,33(7):75.

[7] FLOREA A M. DNA Methylation pyrosequencing assay is applicable for the assessment of epigenetic active environmental or clinical relevant chemicals[J]. Biomed Res Internat,2013,(8):491-512.

[8] RONAGHI M. Pyrosequencing sheds light on DNA sequencing [J]. Genome Res,2001,11(1):3-11.

[9] DUAN H,HE Z,MA J,et al. Global and MGMT promoter hypomethylation independently associated with genomic instability of lymphocytes in subjects exposed to high-dose polycyclic aromatic hydrocarbon[J]. Arch Toxicol,2013,87(11):2013-2022.

[10] HE Z N,DUAN H W,ZHANG B A,et al. CpG site-specific RASSF1a hypermethylation is associated with occupational PAH exposure and genomic instability[J]. Toxicol Res,2015,4(4):848-857.

[11] SHAMES D S,MINNA J D,GAZDAR A F. Methods for detecting DNA methylation in tumors:From bench to bedside [J]. Cancer Letters,2007,251(2):187-198.

[12] RAND K,QU W J,HO T,et al. Conversion-specific detection of DNA methylation using real-time polymerase chain reaction (ConLight-MSP) to avoid false positives[J]. Methods,2002,27(2):114-120.

[13] BRISOTTO G,DI GENNARO A,DAMIANO V,et al. An improved sequencing-based strategy to estimate locus-specific DNA methylation[J]. BMC Cancer,2015,15(1):639-649.

[14] ALEGRIA-TORRES J A,BARRETTA F,BATRES-ESQUIVEL L E,et al. Epigenetic markers of exposure to polycyclic aromatic hydrocarbons in Mexican brickmakers:A pilot study[J]. Chemosphere,2013,91(4):475-480.

[15] KILE M L,FANG S N,BACCARELLI A A,et al. A panel study of occupational exposure to fine particulate matter and changes in DNA methylation over a single workday and years worked in boilermaker welders[J]. Environ Health,2013,12:251-264.

[16] HOU L F,ZHANG X,TARANTINI L,et al. Ambient PM exposure and DNA methylation in tumor suppressor genes:a cross-sectional study[J]. Part and Fibre Toxicol,2011,8(3):280-283.

[17] BRUNET A,BERGER S L. Epigenetics of aging and aging-related disease[J]. J Gerontol A Biol Sci Med Sci,2014,69(Sup 1):17-20.

环境化学污染物暴露相关基因甲基化焦磷酸测序方法的构建和应用

Construction of an environmental pollution-responsive gene-specific pyrosequencing assay

PDF

可视化

摘要/Abstract

引用本文

使用本文

参考文献

相关文章 15

编辑推荐

Metrics

本文评价

[1]	田雪蕾, 封江彬, 田梅, 刘青杰. 甲基化芯片检测电离辐射诱导人外周血淋巴细胞DNA甲基化水平的变化[J]. 癌变·畸变·突变, 2019, 31(6): 434-439.
[2]	彭长凤, 谢杏, 柯跃斌. 纳米氧化石墨烯诱导人类支气管上皮细胞DNA氧化与甲基化的实验研究[J]. 癌变·畸变·突变, 2019, 31(6): 454-458,463.
[3]	吴德生, 杨飞, 袁建辉, 杨淋清, 黄海燕, 刘建军, 庄志雄. PM2.5对斑马鱼胚胎发育早期氧化应激和DNA甲基化调控相关基因表达的影响[J]. 癌变·畸变·突变, 2017, 29(5): 379-382.
[4]	王治, 凌曦, 张国伟, 高建芳, 邹鹏, 井澈, 林哲韬, 刘晋祎, 曹佳, 敖琳. 叶酸对1,3-丁二烯诱发的小鼠DNA低甲基化和染色体损伤的影响[J]. 癌变·畸变·突变, 2017, 29(3): 189-193.
[5]	刘海龙, 高玮, 古盼, 邓燕霞, 黄新凤, 吴德生, 刘建军, 黄海燕. BaP诱导细胞恶性转化过程中DNA甲基化水平的变化[J]. 癌变·畸变·突变, 2017, 29(1): 42-45,50.
[6]	赖怡, 陈佳红, 张航, 乐聪, 姜岩, 陈涛. 丙烯酰胺对F344大鼠肝毒性的分子机制研究[J]. 癌变·畸变·突变, 2016, 28(3): 174-178.
[7]	封杰, 刘文斌, 陈洪强, 黄永胜, 韩飞, 曹佳, 刘晋祎. 肺癌患者MPDZ基因异常甲基化的研究[J]. 癌变·畸变·突变, 2015, 27(6): 437-440.
[8]	赵欢, 刘文斌, 陈洪强, 韩飞, 曹佳, 刘晋祎. TMEM196基因在肺癌中的甲基化修饰与表达调控[J]. 癌变·畸变·突变, 2015, 27(5): 353-356.
[9]	刘耀娴, 倪娟, 周滔, 梁子卿, 汪旭. microRNAs对一碳单位代谢的调控及相应生物学过程的影响[J]. 癌变·畸变·突变, 2015, 27(4): 319-322.
[10]	史荣辉, 韩飞, 董严, 张明谦, 姜晓, 尹俐, 刘文斌, 曹佳, 刘晋祎. SOX30基因在结直肠癌中的表达与甲基化分析[J]. 癌变·畸变·突变, 2015, 27(3): 168-171,176.
[11]	陈佳红, 张航, 赖怡, 姜岩, 陈涛. 三氯乙烯对B6C3F1雄性小鼠肝脏和肾脏中细胞增殖相关基因表达和DNA甲基化的影响[J]. 癌变·畸变·突变, 2015, 27(3): 211-215.
[12]	李金慧，张波，朱伟. DNA甲基化分析方法及相关应用[J]. 癌变·畸变·突变, 2014, 26(4): 313-316.
[13]	陈艳，邓彦超，李磊. 利用甲基化芯片及转录组测序方法筛选哈萨克族食管癌DNA异常甲基化谱[J]. 癌变·畸变·突变, 2014, 26(2): 94-99.
[14]	邓婷婷，谢妮，黄艳华，黄海燕，李子刚，胡章立，袁建辉. 毛细管电泳法检测耐米托蒽醌乳腺癌细胞系全基因组甲基化水平[J]. 癌变·畸变·突变, 2014, 26(2): 108-112.
[15]	柯跃斌，黄娟，朱舟，吴双，陶功华. 甲醛对人Ⅱ型肺泡上皮细胞DNA氧化和甲基化水平的影响[J]. 癌变·畸变·突变, 2014, 26(1): 25-29.