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Mir-29b Mediates the Neural Tube versus Neural Crest Fate Decision during Embryonic Stem Cell Neural Differentiation
Author(s) -
Jiajie Xi,
Yukang Wu,
Guoping Li,
Li Ma,
Ke Feng,
Xudong Guo,
Wenwen Jia,
Guiying Wang,
Guang Yang,
Ping Li,
Jiuhong Kang
Publication year - 2017
Publication title -
stem cell reports
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 3.207
H-Index - 76
ISSN - 2213-6711
DOI - 10.1016/j.stemcr.2017.06.017
Subject(s) - neural crest , biology , embryonic stem cell , neural tube , neural plate , microbiology and biotechnology , neural stem cell , cellular differentiation , neuroectoderm , neural development , microrna , neural cell , stem cell , cancer research , mesoderm , cell , genetics , embryo , gene
During gastrulation, the neuroectoderm cells form the neural tube and neural crest. The nervous system contains significantly more microRNAs than other tissues, but the role of microRNAs in controlling the differentiation of neuroectodermal cells into neural tube epithelial (NTE) cells and neural crest cells (NCCs) remains unknown. Using embryonic stem cell (ESC) neural differentiation systems, we found that miR-29b was upregulated in NTE cells and downregulated in NCCs. MiR-29b promoted the differentiation of ESCs into NTE cells and inhibited their differentiation into NCCs. Accordingly, the inhibition of miR-29b significantly inhibited the differentiation of NTE cells. A mechanistic study revealed that miR-29b targets DNA methyltransferase 3a (Dnmt3a) to regulate neural differentiation. Moreover, miR-29b mediated the function of Pou3f1, a critical neural transcription factor. Therefore, our study showed that the Pou3f1-miR-29b-Dnmt3a regulatory axis was active at the initial stage of neural differentiation and regulated the determination of cell fate.

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