Literature DB >> 34919141

Regulation of retinal amacrine cell generation by miR-216b and Foxn3.

Huanqing Zhang1, Pei Zhuang1, Ryan M Welchko1, Manhong Dai1, Fan Meng1,2, David L Turner1,3.   

Abstract

The mammalian retina contains a complex mixture of different types of neurons. We find that microRNA miR-216b is preferentially expressed in postmitotic retinal amacrine cells in the mouse retina, and expression of miR-216a/b and miR-217 in retina depend in part on Ptf1a, a transcription factor required for amacrine cell differentiation. Surprisingly, ectopic expression of miR-216b directed the formation of additional amacrine cells and reduced bipolar neurons in the developing retina. We identify the Foxn3 mRNA as a retinal target of miR-216b by Argonaute PAR-CLIP and reporter analysis. Inhibition of Foxn3, a transcription factor, in the postnatal developing retina by RNAi increased the formation of amacrine cells and reduced bipolar cell formation. Foxn3 disruption by CRISPR in embryonic retinal explants also increased amacrine cell formation, whereas Foxn3 overexpression inhibited amacrine cell formation prior to Ptf1a expression. Co-expression of Foxn3 partially reversed the effects of ectopic miR-216b on retinal cell formation. Our results identify Foxn3 as a novel regulator of interneuron formation in the developing retina and suggest that miR-216b likely regulates Foxn3 and other genes in amacrine cells.
© 2022. Published by The Company of Biologists Ltd.

Entities:  

Keywords:  Cell fate; Neurogenesis; Retina; microRNA

Mesh:

Substances:

Year:  2022        PMID: 34919141      PMCID: PMC8917416          DOI: 10.1242/dev.199484

Source DB:  PubMed          Journal:  Development        ISSN: 0950-1991            Impact factor:   6.868


  93 in total

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