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Integrated detection of both 5-mC and 5-hmC by high-throughput tag sequencing technology highlights methylation reprogramming of bivalent genes during cellular differentiation

  • Fei Gao
  • , Yudong Xia
  • , Junwen Wang
  • , Huijuan Luo
  • , Zhaowei Gao
  • , Xu Han
  • , Juyong Zhang
  • , Xiaojun Huang
  • , Yu Yao
  • , Hanlin Lu
  • , Na Yi
  • , Baojin Zhou
  • , Zhilong Lin
  • , Bo Wen
  • , Xiuqing Zhang
  • , Huanming Yang
  • , Jun Wang

科研成果: 期刊稿件文章同行评审

30 引用 (Scopus)

摘要

5-methylcytosine (5-mC) can be oxidized to 5-hydroxymethylcytosine (5-hmC). Genome-wide profiling of 5-hmC thus far indicates 5-hmC may not only be an intermediate form of DNA demethylation but could also constitute an epigenetic mark per se. Here we describe a cost-effective and selective method to detect both the hydroxymethylation and methylation status of cytosines in a subset of cytosines in the human genome. This method involves the selective glucosylation of 5-hmC residues, short-sequence tag generation and high-throughput sequencing. We tested this method by screening H9 human embryonic stem cells and their differentiated embroid body cells, and found that differential hydroxymethylation preferentially occurs in bivalent genes during cellular differentiation. Especially, our results support hydroxymethylation can regulate key transcription regulators with bivalent marks through demethylation and affect cellular decision on choosing active or inactive state of these genes upon cellular differentiation. Future application of this technology would enable us to uncover the status of methylation and hydroxymethylation in dynamic biological processes and disease development in multiple biological samples.

源语言英语
期刊Epigenetics
8
4
DOI
出版状态已出版 - 4月 2013
已对外发布

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