4.8 Article

Regulatory Dynamics of Tet1 and Oct4 Resolve Stages of Global DNA Demethylation and Transcriptomic Changes in Reprogramming

Journal

CELL REPORTS
Volume 30, Issue 7, Pages 2150-2169

Publisher

CELL PRESS
DOI: 10.1016/j.celrep.2020.01.065

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Funding

  1. Belgium Research Foundation -Flanders (FWO) [G.0C56.13N, G0F7716N, G.0632.13]
  2. Ministerie van de Vlaamse Gemeenschap
  3. European Commission FP7-PEOPLE-2012-CIG Career Integration Grant [321658]
  4. KU Leuven Internal Funds [C14/16/077]
  5. SCIL program
  6. FWO PhD fellowships [11E7920N, 1158318N]
  7. China Scholarship Council
  8. Taiwan Ministry of Education (MOE)-KU Leuven PhD scholarship

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Reprogramming somatic cells into induced pluripotent stem cells (iPSCs) involves the reactivation of endogenous pluripotency genes and global DNA demethylation, but temporal resolution of these events using existing markers is limited. Here, we generate murine transgenic lines harboring reporters for the 5-methylcytosine dioxygenase Tet1 and for Oct4. By monitoring dual reporter fluorescence during pluripotency entry, we identify a sequential order of Tet1 and Oct4 activation by proximal and distal regulatory elements. Full Tet1 activation marks an intermediate stage that accompanies predominantly repression of somatic genes, preceding full Oct4 activation, and distinguishes two waves of global DNA demethylation that target distinct genomic features but are uncoupled from transcriptional changes. Tet1 knockout shows that TET1 contributes to both waves of demethylation and activates germline regulatory genes in reprogramming intermediates but is dispensable for Oct4 reactivation. Our dual reporter system for time-resolving pluripotency entry thus refines the molecular roadmap of iPSC maturation.

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