Canonical microRNAs Enable Differentiation, Protect Against DNA Damage, and Promote Cholesterol Biosynthesis in Neural Stem Cells

Liu, Zhong; Zhang, Cheng; Khodadadi‐Jamayran, Alireza; Dang, Lam; Han, Xiaosi; Kim, Kitai; Li, Hu; Zhao, Rui

doi:10.1089/scd.2016.0259

Cited by 10 publications

(13 citation statements)

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“…Taken together, this evidence indicates that DGCR8 promotes cortical NPC self-renewal and represses their differentiation in vivo , possibly by a cell-autonomous function. Our results are consistent with previous observations in mouse ESCs (Wang et al, 2007 ; Cirera-Salinas et al, 2017a , b ) and NPCs in vitro (Liu et al, 2017 ). Of note, overexpression of DGCR8 at later developmental stages (i.e., when upper cortical layer neurons are generated) selectively promotes expansion of BPs (Figure 5 ), opening intriguing perspectives for a DGCR8-dependent control in the radial neocortex enlargement in evolution, which reflects a striking increase in BP population and upper cortical layers size (Fietz and Huttner, 2011 ; Reillo et al, 2011 ; Shitamukai et al, 2011 ; Wang et al, 2011 ; Borrell and Reillo, 2012 ; Hevner and Haydar, 2012 ; Kelava et al, 2012 ; Betizeau et al, 2013 ; LaMonica et al, 2013 ).…”

Section: Discussionsupporting

confidence: 94%

DGCR8 Promotes Neural Progenitor Expansion and Represses Neurogenesis in the Mouse Embryonic Neocortex

et al. 2018

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DGCR8 and DROSHA are the minimal functional core of the Microprocessor complex essential for biogenesis of canonical microRNAs and for the processing of other RNAs. Conditional deletion of Dgcr8 and Drosha in the murine telencephalon indicated that these proteins exert crucial functions in corticogenesis. The identification of mechanisms of DGCR8- or DROSHA-dependent regulation of gene expression in conditional knockout mice are often complicated by massive apoptosis. Here, to investigate DGCR8 functions on amplification/differentiation of neural progenitors cells (NPCs) in corticogenesis, we overexpress Dgcr8 in the mouse telencephalon, by in utero electroporation (IUEp). We find that DGCR8 promotes the expansion of NPC pools and represses neurogenesis, in absence of apoptosis, thus overcoming the usual limitations of Dgcr8 knockout-based approach. Interestingly, DGCR8 selectively promotes basal progenitor amplification at later developmental stages, entailing intriguing implications for neocortical expansion in evolution. Finally, despite a 3- to 5-fold increase of DGCR8 level in the mouse telencephalon, the composition, target preference and function of the DROSHA-dependent Microprocessor complex remain unaltered. Thus, we propose that DGCR8-dependent modulation of gene expression in corticogenesis is more complex than previously known, and possibly DROSHA-independent.

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Section: Discussionsupporting

confidence: 94%

DGCR8 Promotes Neural Progenitor Expansion and Represses Neurogenesis in the Mouse Embryonic Neocortex

et al. 2018

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“…Collected cells were washed twice with serumless DMEM/F12 (300×G, 7 minutes, 4°C), counted in the presence of 0.04% trypan blue to enumerate viable cells. Dissociated LGG cells were cultured in cell culture plates coated with poly-L-ornithine (Sigma-Aldrich) and laminin (EMD-Millipore) in LGG medium (Neurobasal-A medium containing 1% N-2, 2% vitamin A-free B-27, 2 mM L-Glutamine [Thermo Fisher], 20 ng/ml basic FGF [Stemgent], and 20 ng/ml human EGF [Cell Signaling]) as described [15,16]. Medium was exchanged as needed, and cells grew adherently to the bottom of flasks.…”

Section: Methodsmentioning

confidence: 99%

“…For immunostaining, iPSCs were fixed in 4% PFA, blocked in Protein Block (Agilent), stained with primary antibodies at 4 °C overnight and secondary antibodies at room temperature for 1 hour as described [15,25]. Primary antibodies used were OCT4 (sc-5279, Santa Cruz Biotech), SOX2 (561469, BD Biosciences), and NANOG (AF1977, R&D Systems).…”

Section: Methodsmentioning

confidence: 99%

Characterization of iPSCs derived from low grade gliomas revealed early regional chromosomal amplifications during gliomagenesis

et al. 2018

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Introduction. IDH1 mutation has been identified as a early genetic event driving low grade gliomas (LGGs) and it has been proven to exerts a powerful epigenetic effect. Cells containing IDH1 mutation are refractory to epigenetical reprogramming to iPSC induced by expression of Yamanaka transcription factors, a feature that we employed to study early genetic amplifications or deletions in gliomagenesis. Methods. We made iPSC clones from freshly surgically resected IDH1 mutant LGGs by forced expression of Yamanaka transcription factors. We sequenced the IDH locus and analyzed the genetic composition of multiple iPSC clones by array-based comparative genomic hybridization (aCGH). Results. We hypothesize that the primary cell pool isolated from LGG tumor contains a heterogeneous population consisting tumor cells at various stages of tumor progression including cells with early genetic lesions if any prior to acquisition of IDH1 mutation. Because cells containing IDH1 mutation are refractory to reprogramming, we predict that iPSC clones should originate only from LGG cells without IDH1 mutation, i.e. cells prior to acquisition of IDH1 mutation. As expected, we found that none of the iPSC clones contains IDH1 mutation. Further analysis by aCGH of the iPCS clones reveals that they contain regional chromosomal amplifications which are also present in the primary LGG cells. Conclusions. These results indicate that there exists a subpopulation of cells harboring gene amplification but without IDH1 mutation in the LGG primary cell pool. Further analysis of TCGA LGG database demonstrates that these regional chromosomal amplifications are also present in some cases of low grade gliomas indicating they are reoccurring lesions in glioma albeit at a low frequency. Taken together, these data suggest that regional chromosomal alterations may exist prior to the acquisition of IDH mutations in at least some cases of LGGs.

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“…Immunostaining was performed as described previously ( Liu et al., 2017 ). In brief, EBs were fixed in 4% paraformaldehyde, blocked in Protein Block (Dako), and incubated with the appropriate primary antibodies overnight at 4°C and secondary antibodies for 1 hr at room temperature.…”

Section: Methodsmentioning

confidence: 99%

“…Cells were analyzed on a BD Fortessa flow cytometer. Apoptosis analysis was performed as described previously ( Liu et al., 2017 ). In brief, ESCs were treated with the indicated concentration of nutlin-3a or 50 ng/mL NCS (Sigma-Aldrich) for 24 hr.…”

Section: Methodsmentioning

confidence: 99%

Elevated p53 Activities Restrict Differentiation Potential of MicroRNA-Deficient Pluripotent Stem Cells

et al. 2017

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SummaryPluripotent stem cells (PSCs) deficient for microRNAs (miRNAs), such as Dgcr8−/− or Dicer−/– embryonic stem cells (ESCs), contain no mature miRNA and cannot differentiate into somatic cells. How miRNA deficiency causes differentiation defects remains poorly understood. Here, we report that miR-302 is sufficient to enable neural differentiation of differentiation-incompetent Dgcr8−/− ESCs. Our data showed that miR-302 directly suppresses the tumor suppressor p53, which is modestly upregulated in Dgcr8−/− ESCs and serves as a barrier restricting neural differentiation. We demonstrated that direct inactivation of p53 by SV40 large T antigen, a short hairpin RNA against Trp53, or genetic ablation of Trp53 in Dgcr8−/− PSCs enables neural differentiation, while activation of p53 by the MDM2 inhibitor nutlin-3a in wild-type ESCs inhibits neural differentiation. Together, we demonstrate that a major function of miRNAs in neural differentiation is suppression of p53 and that modest activation of p53 blocks neural differentiation of miRNA-deficient PSCs.

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Canonical microRNAs Enable Differentiation, Protect Against DNA Damage, and Promote Cholesterol Biosynthesis in Neural Stem Cells

Cited by 10 publications

References 58 publications

DGCR8 Promotes Neural Progenitor Expansion and Represses Neurogenesis in the Mouse Embryonic Neocortex

DGCR8 Promotes Neural Progenitor Expansion and Represses Neurogenesis in the Mouse Embryonic Neocortex

Characterization of iPSCs derived from low grade gliomas revealed early regional chromosomal amplifications during gliomagenesis

Elevated p53 Activities Restrict Differentiation Potential of MicroRNA-Deficient Pluripotent Stem Cells

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