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滤泡型甲状腺肿瘤中 DNA 甲基化谱与恶性肿瘤之间的关联。

Association between DNA methylation profile and malignancy in follicular-patterned thyroid neoplasms.

机构信息

Dipartimento di Medicina Molecolare e Biotecnologie Mediche, Università Federico II, Napoli, Italy.

Istituto di Endocrinologia ed Oncologia Sperimentale, Consiglio Nazionale delle Ricerche, Napoli, Italy.

出版信息

Endocr Relat Cancer. 2019 Apr 1;26(4):451-462. doi: 10.1530/ERC-18-0308. Epub 2019 Feb 1.

DOI:10.1530/ERC-18-0308
PMID:30753136
Abstract

Molecular differentiation between benign (follicular thyroid adenoma, FTA) and malignant (follicular thyroid carcinoma, FTC) thyroid neoplasms is challenging. Here, we explored the genome-wide DNA methylation profile of FTA (n.10) and FTC (n.11) compared to normal thyroid (NT) (n.7) tissues. FTC featured 3,564 differentially-methylated CpGs (DMCpG), most (84%) of them hypermethylated, with respect to normal controls. At the principal component analysis (PCA), the methylation profile of FTA occupied an intermediate position between FTC and normal tissue. A large fraction (n. 2,385) of FTC-associated DMCpG were related (intragenic or within 1500 bp from the transcription start site) to annotated genes (n. 1,786). FTC-hypermethylated genes were enriched for targets of the Polycomb transcriptional repressor complex and the specific histone H3 marks (H3K4me2/me3-H3K27me3) found in chromatin domains known as "bivalent". Transcriptome profiling by RNAseq showed that 7.9% of the DMCpGs-associated genes were differentially expressed in FTC compared to NT, suggesting that altered DNA methylation may contribute to their altered expression. Overall, this study suggests that perturbed DNA methylation, in particular hypermethylation, is a component of the molecular mechanisms leading to the formation of FTC and that DNA methylation profiling may help differentiating FTCs from their benign counterpart.

摘要

良性(滤泡状甲状腺腺瘤,FTA)和恶性(滤泡状甲状腺癌,FTC)甲状腺肿瘤之间的分子分化具有挑战性。在这里,我们比较了正常甲状腺(NT)(n=7)组织与 FTA(n=10)和 FTC(n=11)的全基因组 DNA 甲基化谱。FTC 有 3564 个差异甲基化 CpG(DMCpG),与正常对照相比,其中大多数(84%)呈超甲基化。在主成分分析(PCA)中,FTA 的甲基化谱在 FTC 和正常组织之间处于中间位置。FTC 相关的 DMCpG 中有很大一部分(n=2385)与注释基因(n=1786)相关(基因内或转录起始位点 1500bp 内)。FTC 超甲基化基因富集了多梳转录抑制复合物和特定组蛋白 H3 标记(H3K4me2/me3-H3K27me3)的靶标,这些标记存在于已知的“双价”染色质域中。RNAseq 转录组分析显示,在 FTC 与 NT 相比,7.9%的 DMCpG 相关基因表达存在差异,这表明 DNA 甲基化的改变可能导致其表达的改变。总的来说,这项研究表明,失调的 DNA 甲基化,特别是超甲基化,是导致 FTC 形成的分子机制的一部分,DNA 甲基化谱分析可能有助于区分 FTC 与其良性 counterpart。

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