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整合高分辨率甲基化组和转录组分析,解析儿童急性淋巴细胞白血病中的表观基因组变化。

Integration of high-resolution methylome and transcriptome analyses to dissect epigenomic changes in childhood acute lymphoblastic leukemia.

机构信息

Department of Human Genetics, McGill University, Montréal, Canada.

出版信息

Cancer Res. 2013 Jul 15;73(14):4323-36. doi: 10.1158/0008-5472.CAN-12-4367. Epub 2013 May 30.

DOI:10.1158/0008-5472.CAN-12-4367
PMID:23722552
Abstract

B-cell precursor acute lymphoblastic leukemia (pre-B ALL) is the most common pediatric cancer. Although the genetic determinants underlying disease onset remain unclear, epigenetic modifications including DNA methylation are suggested to contribute significantly to leukemogenesis. Using the Illumina 450K array, we assessed DNA methylation in matched tumor-normal samples of 46 childhood patients with pre-B ALL, extending single CpG-site resolution analysis of the pre-B ALL methylome beyond CpG-islands (CGI). Unsupervised hierarchical clustering of CpG-site neighborhood, gene, or microRNA (miRNA) gene-associated methylation levels separated the tumor cohort according to major pre-B ALL subtypes, and methylation in CGIs, CGI shores, and in regions around the transcription start site was found to significantly correlate with transcript expression. Focusing on samples carrying the t(12;21) ETV6-RUNX1 fusion, we identified 119 subtype-specific high-confidence marker CpG-loci. Pathway analyses linked the CpG-loci-associated genes with hematopoiesis and cancer. Further integration with whole-transcriptome data showed the effects of methylation on expression of 17 potential drivers of leukemogenesis. Independent validation of array methylation and sequencing-derived transcript expression with Sequenom Epityper technology and real-time quantitative reverse transcriptase PCR, respectively, indicates more than 80% empirical accuracy of our genome-wide findings. In summary, genome-wide DNA methylation profiling enabled us to separate pre-B ALL according to major subtypes, to map epigenetic biomarkers specific for the t(12;21) subtype, and through a combined methylome and transcriptome approach to identify downstream effects on candidate drivers of leukemogenesis.

摘要

B 细胞前体急性淋巴细胞白血病 (pre-B ALL) 是最常见的儿科癌症。尽管疾病发生的遗传决定因素尚不清楚,但包括 DNA 甲基化在内的表观遗传修饰被认为对白血病的发生有重要贡献。我们使用 Illumina 450K 阵列评估了 46 例儿童 pre-B ALL 患者配对肿瘤-正常样本中的 DNA 甲基化,扩展了 pre-B ALL 甲基组中单 CpG 位点分辨率分析超出 CpG 岛 (CGI) 的范围。CpG 位点邻域、基因或 microRNA (miRNA) 基因相关甲基化水平的无监督层次聚类根据主要 pre-B ALL 亚型分离了肿瘤队列,并且 CGI、CGI 岸和转录起始位点周围区域的甲基化与转录物表达显著相关。我们关注携带 t(12;21) ETV6-RUNX1 融合的样本,鉴定了 119 个亚型特异性高置信标记 CpG 位点。通路分析将 CpG 位点相关基因与造血和癌症联系起来。与全转录组数据的进一步整合表明,甲基化对 17 个潜在白血病发生驱动基因的表达有影响。使用 Sequenom Epityper 技术分别对芯片甲基化和测序衍生的转录物表达进行独立验证,以及实时定量逆转录 PCR,分别表明我们全基因组发现的经验准确性超过 80%。总之,全基因组 DNA 甲基化谱分析使我们能够根据主要亚型对 pre-B ALL 进行分类,绘制特定于 t(12;21) 亚型的表观遗传生物标志物,并通过甲基组和转录组联合方法鉴定对白血病发生的候选驱动基因的下游影响。

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