AI Article Synopsis

  • - Researchers focused on miR-124, a non-coding RNA, to understand its role in neuronal differentiation and its complex regulation of various biological processes during neurogenesis.
  • - They utilized CRISPR/Cas9 technology to delete all six miR-124 alleles in human stem cells, leading to the formation of functional neurons with changed structure and neurotransmitter types.
  • - By identifying 98 key targets of miR-124 and analyzing their effects on cell viability and neuronal characteristics, the study highlighted the importance of combining experimental and systemic approaches to fully understand miRNA roles in human brain neurogenesis.

Article Abstract

Non-coding RNAs regulate many biological processes including neurogenesis. The brain-enriched miR-124 has been assigned as a key player of neuronal differentiation via its complex but little understood regulation of thousands of annotated targets. To systematically chart its regulatory functions, we used CRISPR/Cas9 gene editing to disrupt all six miR-124 alleles in human induced pluripotent stem cells. Upon neuronal induction, miR-124-deleted cells underwent neurogenesis and became functional neurons, albeit with altered morphology and neurotransmitter specification. Using RNA-induced-silencing-complex precipitation, we identified 98 high-confidence miR-124 targets, of which some directly led to decreased viability. By performing advanced transcription-factor-network analysis, we identified indirect miR-124 effects on apoptosis, neuronal subtype differentiation, and the regulation of previously uncharacterized zinc finger transcription factors. Our data emphasize the need for combined experimental- and system-level analyses to comprehensively disentangle and reveal miRNA functions, including their involvement in the neurogenesis of diverse neuronal cell types found in the human brain.

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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC6205824PMC
http://dx.doi.org/10.1016/j.cels.2018.08.011DOI Listing

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