DOT1L activity affects neural stem cell division mode and reduces differentiation and ASNS expression.
Bismark AppiahCamila L FullioChiara OssolaIlaria BertaniElena RestelliArquimedes ChefferMartina PolenghiChristiane HaffnerMarta Garcia-MirallesPatrice ZeisMartin TreppnerPatrick BovioLaura SchlichtholzAina Mas-SanchezLea ZografidouJennifer WinterHarald BinderDominic GrünNereo KalebicElena TavernaTanja VogelPublished in: EMBO reports (2023)
Cortical neurogenesis depends on the balance between self-renewal and differentiation of apical progenitors (APs). Here, we study the epigenetic control of AP's division mode by focusing on the enzymatic activity of the histone methyltransferase DOT1L. Combining lineage tracing with single-cell RNA sequencing of clonally related cells, we show at the cellular level that DOT1L inhibition increases neurogenesis driven by a shift of APs from asymmetric self-renewing to symmetric neurogenic consumptive divisions. At the molecular level, DOT1L activity prevents AP differentiation by promoting transcription of metabolic genes. Mechanistically, DOT1L inhibition reduces activity of an EZH2/PRC2 pathway, converging on increased expression of asparagine synthetase (ASNS), a microcephaly associated gene. Overexpression of ASNS in APs phenocopies DOT1L inhibition, and also increases neuronal differentiation of APs. Our data suggest that DOT1L activity/PRC2 crosstalk controls AP lineage progression by regulating asparagine metabolism.
Keyphrases
- single cell
- stem cells
- transcription factor
- energy transfer
- dna methylation
- genome wide
- poor prognosis
- rna seq
- induced apoptosis
- zika virus
- mesenchymal stem cells
- high throughput
- oxidative stress
- nitric oxide
- machine learning
- signaling pathway
- spinal cord injury
- binding protein
- brain injury
- cell cycle arrest
- solid state
- cell fate