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定量评估炎症型和非炎症型乳腺癌表型中的 DNA 高甲基化。

Quantitative assessment of DNA hypermethylation in the inflammatory and non-inflammatory breast cancer phenotypes.

机构信息

Translational Cancer Research Group, Laboratory of Pathology, University of Antwerp/University Hospital Antwerp, Oncology Centre, General Hospital St-Augustinus, Antwerp, Belgium.

出版信息

Cancer Biol Ther. 2009 Dec;8(23):2252-9. doi: 10.4161/cbt.8.23.10133. Epub 2009 Dec 19.

Abstract

In this study, a comparative quantitative methylation profiling of inflammatory breast cancer (IBC) and non-IBC was set up for the identification of tumor-specific methylation patterns. Methylation ratios of six genes (DAPK, TWIST, HIN-1, RASSF1A, RARbeta2 and APC) were measured in benign breast tissues (n = 9) and in tumor samples from non-IBC (n = 81) and IBC (n = 19) patients using quantitative methylation-specific PCR. Median methylation ratios observed in breast cancer (n = 100) were significantly higher than those observed in benign breast tissues for five of six genes (TWIST, HIN-1, RASSF1A, RARbeta2 and APC). Only one of the individual genes studied, RARbeta2, showed differential methylation ratios in IBC and non-IBC (p = 0.016). Using the maximal methylation ratio observed in benign breast tissue as a threshold, the methylation frequency of two genes, RARbeta2 and APC, was significantly increased in IBC (n = 19) when compared to non-IBC (n = 81): 53 vs. 23% for RARbeta2 (p = 0.012) and 84 vs. 54% for APC (p = 0.017). Using hierarchical clustering, methylation patterns could not classify breast cancers according to their phenotype. The finding of differential frequencies of methylation in IBC and non-IBC for two out of six genes suggests that gene-specific patterns of methylation could provide a basis for molecular classification of IBC. Testing for additional genes could help to define the IBC phenotype based on patterns of aberrant gene promoter methylation.

摘要

在这项研究中,我们建立了一个比较炎症性乳腺癌(IBC)和非 IBC 的定量甲基化分析,以鉴定肿瘤特异性的甲基化模式。采用定量甲基化特异性 PCR 法检测 6 个基因(DAPK、TWIST、HIN-1、RASSF1A、RARβ2 和 APC)在良性乳腺组织(n=9)和非 IBC (n=81)及 IBC (n=19)肿瘤样本中的甲基化比率。在乳腺癌(n=100)中观察到的中位数甲基化比率明显高于良性乳腺组织中观察到的五个基因(TWIST、HIN-1、RASSF1A、RARβ2 和 APC)。在所研究的单个基因中,只有一个基因 RARβ2 在 IBC 和非 IBC 中显示出不同的甲基化比率(p=0.016)。使用良性乳腺组织中观察到的最大甲基化比率作为阈值,两个基因(RARβ2 和 APC)的甲基化频率在 IBC(n=19)中明显高于非 IBC(n=81):RARβ2 为 53%比 23%(p=0.012),APC 为 84%比 54%(p=0.017)。通过层次聚类,甲基化模式不能根据乳腺癌的表型对其进行分类。在 IBC 和非 IBC 中,有两个基因(RARβ2 和 APC)的甲基化频率存在差异,这表明基因特异性的甲基化模式可能为 IBC 的分子分类提供基础。对其他基因的检测可能有助于根据异常基因启动子甲基化模式定义 IBC 表型。

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