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首页> 外文期刊>International Journal of Cancer =: Journal International du Cancer >Promoter DNA hypermethylation in gastric biopsies from subjects at high and low risk for gastric cancer.
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Promoter DNA hypermethylation in gastric biopsies from subjects at high and low risk for gastric cancer.

机译:胃癌高风险和低风险受试者的胃活检中的DNA甲基化促进子。

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Gene promoter CpG island hypermethylation is associated with Helicobacter pylori (H. pylori) infection and may be an important initiator of gastric carcinogenesis. To examine factors influencing methylation, we utilized bisulfite Pyrosequencing(R) technology for quantitative analysis of promoter DNA methylation in RPRM, APC, MGMT and TWIST1 genes using DNA from 86 gastric biopsies from Colombian residents of areas with high and low incidence of gastric cancer. H. pylori colonies were cultured from the same subjects, and gastric pathology was evaluated. Virulence factors cagA (including segments of the 3' end, encoding EPIYA polymorphisms) and vacA s and m regions were characterized in the H. pylori strains. Using univariate analysis, we found significantly elevated levels of RPRM and TWIST1 promoter DNA methylation in biopsies from residents of the high-risk region compared to those from residents of the low-risk region. The presence of cagA and vacA s1m1 alleles were independently associated with elevated levels of promoter DNA methylation of RPRM and MGMT. Using multivariate analysis, DNA methylation of RPRM was associated with location of residence, cagA and vacA s1m1 status and methylation of TWIST1. We conclude that cagA and vacA virulence determinants are significantly associated with quantitative differences in promoter DNA methylation in these populations, but that other as yet undefined factors that differ between the populations may also contribute to variation in methylation status.
机译:基因启动子CpG岛甲基化与幽门螺杆菌(H. pylori)感染有关,可能是胃癌发生的重要引发剂。为了检查影响甲基化的因素,我们使用了亚硫酸氢盐测序技术,对来自哥伦比亚高发地区和低发地区的86名胃活检组织中的RPRM,APC,MGMT和TWIST1基因中的启动子DNA甲基化进行了定量分析。从同一受试者培养幽门螺杆菌菌落,并评估胃病理学。在幽门螺杆菌菌株中鉴定了毒力因子cagA(包括3'末端的片段,编码EPIRA多态性)和vacA s和m区域。使用单变量分析,我们发现与高危地区居民相比,高危地区居民活检中的RPRM和TWIST1启动子DNA甲基化水平显着升高。 cagA和vacA s1m1等位基因的存在与RPRM和MGMT启动子DNA甲基化水平的升高独立相关。使用多变量分析,RPRM的DNA甲基化与居住位置,cagA和vacA s1m1状态以及TWIST1的甲基化相关。我们得出的结论是,在这些人群中,cagA和vacA毒力决定因素与启动子DNA甲基化的数量差异显着相关,但是在人群之间不同的其他尚未定义的因素也可能导致甲基化状态的变化。

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