FoxO3 regulates neuronal reprogramming of cells from postnatal and aging mice

Ahlenius, Henrik; Chanda, Soham; Webb, Ashley E.; Yousif, Issa; Karmazin, Jesse; Prusiner, Stanley B.; Brunet, Anne; Südhof, Thomas C.; Wernig, Marius

doi:10.1073/pnas.1607079113

Cited by 25 publications

(14 citation statements)

References 26 publications

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“…Our analysis found that individuals with nonsynonymous variants in FOXO3 had lower HbF levels. FOXO3 is a transcription factor that has been shown to be essential for erythroid maturation in mouse models, 22,24 and it is an important regulator of glucose metabolism, 17,60,61 among other functions 14,[62][63][64][65][66] ; however, it has not previously been implicated in HbF regulation. Here, we presented functional studies supporting the hypothesis that FOXO3 is a partial positive regulator of HbF, likely along with other factors; knockdown of FOXO3 in HSPCs from normal individuals reduced g-globin expression and production without altering b-globin expression and production.…”

Section: Discussionmentioning

confidence: 99%

Metformin induces FOXO3-dependent fetal hemoglobin production in human primary erythroid cells

Zhang

Paikari

Sumazin

et al. 2018

Blood

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Induction of red blood cell (RBC) fetal hemoglobin (HbF; α2γ2) ameliorates the pathophysiology of sickle cell disease (SCD) by reducing the concentration of sickle hemoglobin (HbS; α2β2) to inhibit its polymerization. Hydroxyurea (HU), the only US Food and Drug Administration (FDA)-approved drug for SCD, acts in part by inducing HbF; however, it is not fully effective, reflecting the need for new therapies. Whole-exome sequence analysis of rare genetic variants in SCD patients identified as a candidate regulator of RBC HbF. We validated these genomic findings through loss- and gain-of-function studies in normal human CD34 hematopoietic stem and progenitor cells induced to undergo erythroid differentiation. gene silencing reduced γ-globin RNA levels and HbF levels in erythroblasts, whereas overexpression of FOXO3 produced the opposite effect. Moreover, treatment of primary CD34 cell-derived erythroid cultures with metformin, an FDA-approved drug known to enhance FOXO3 activity in nonerythroid cells, caused dose-related FOXO3-dependent increases in the percentage of HbF protein and the fraction of HbF-immunostaining cells (F cells). Combined HU and metformin treatment induced HbF additively and reversed the arrest in erythroid maturation caused by HU treatment alone. HbF induction by metformin in erythroid precursors was dependent on FOXO3 expression and did not alter expression of BCL11A, MYB, or KLF1. Collectively, our data implicate FOXO3 as a positive regulator of γ-globin expression and identify metformin as a potential therapeutic agent for SCD.

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Section: Discussionmentioning

confidence: 99%

Metformin induces FOXO3-dependent fetal hemoglobin production in human primary erythroid cells

Zhang

Paikari

Sumazin

et al. 2018

Blood

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“…GFP-tagged miNSCs or hiNSCs (1 × 10 5 ) were plated on the glial cell feeder with NSC medium in a well of 24-well plate. To optimize the differentiation procedure, 24 h before plating miNSCs or hiNSCs, 3 × 10 4 glial cells were plated as the feeder, which were dissociated from P0 C57BL/6J mouse brain as previous described 80 . After 24 h, the medium was replaced with neuronal differentiation medium 1 (N3 medium supplemented with 2% B27, 1% N2, 2 mM glutamax, and 1 × Pen/Strep), which was replaced with neuronal differentiation medium 2 [neurobasal-a medium supplemented with 1 × Insulin-transferrin-selenium solution (Thermo Fisher), 30 ng/ml BDNF, 30 ng/ml CNTF, 30 ng/ml Nerve growth factor (Pepro Tech), 10 μM forskolin, 25 mM l -glutamic acid, 200 mM l -glutamine, 1% B27, 1% N2, and 1 × Pen/Strep].…”

Section: Methodsmentioning

confidence: 99%

Direct reprogramming of fibroblasts into neural stem cells by single non-neural progenitor transcription factor Ptf1a

Xiao

Liu

Zhang³

et al. 2018

Nat Commun

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Induced neural stem cells (iNSCs) reprogrammed from somatic cells have great potentials in cell replacement therapies and in vitro modeling of neural diseases. Direct conversion of fibroblasts into iNSCs has been shown to depend on a couple of key neural progenitor transcription factors (TFs), raising the question of whether such direct reprogramming can be achieved by non-neural progenitor TFs. Here we report that the non-neural progenitor TF Ptf1a alone is sufficient to directly reprogram mouse and human fibroblasts into self-renewable iNSCs capable of differentiating into functional neurons, astrocytes and oligodendrocytes, and improving cognitive dysfunction of Alzheimer’s disease mouse models when transplanted. The reprogramming activity of Ptf1a depends on its Notch-independent interaction with Rbpj which leads to subsequent activation of expression of TF genes and Notch signaling required for NSC specification, self-renewal, and homeostasis. Together, our data identify a non-canonical and safer approach to establish iNSCs for research and therapeutic purposes.

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“…Further, in some iN studies, the age of the human donor has been negatively correlated with the percentage of iNs obtained [38], and fibroblasts from adult human donors are resistant to Ascl1/Brn2-based conversion, while fetal fibroblasts are highly amenable [38]. RE1-silencing complex (REST), a major neuronal gene repressor in non-neuronal cells, and the aging-associated TF FOXO3 play important roles in controlling neuronal gene expression and show differential activity between fetal and adult/old fibroblasts, resulting in decreased conversion efficacy in aged starting cells [38][39][40]. Again, the combination of the two pioneer factors Ascl1 and Ngn2, for example, fused via a 2A peptide sequence, has yielded iN efficiencies of typically over 50% across large sample sizes and does not appear to be affected by donor age [9,10,35].…”

Section: Enabling In Conversionmentioning

confidence: 99%

Next‐generation disease modeling with direct conversion: a new path to old neurons

2019

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Within just over a decade, human reprogramming-based disease modeling has developed from a rather outlandish idea into an essential part of disease research. While iPSCs are a valuable tool for modeling developmental and monogenetic disorders, their rejuvenated identity poses limitations for modeling age-associated diseases. Direct cell-type conversion of fibroblasts into induced neurons (iNs) circumvents rejuvenation and preserves hallmarks of cellular aging. iNs are thus advantageous for modeling diseases that possess strong age-related and epigenetic contributions and can complement iPSCbased strategies for disease modeling. In this review, we provide an overview of the state of the art of direct iN conversion and describe the key epigenetic, transcriptomic, and metabolic changes that occur in converting fibroblasts. Furthermore, we summarize new insights into this fascinating process, particularly focusing on the rapidly changing criteria used to define and characterize in vitro-born human neurons. Finally, we discuss the unique features that distinguish iNs from other reprogramming-based neuronal cell models and how iNs are relevant to disease modeling.

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FoxO3 regulates neuronal reprogramming of cells from postnatal and aging mice

Cited by 25 publications

References 26 publications

Metformin induces FOXO3-dependent fetal hemoglobin production in human primary erythroid cells

Metformin induces FOXO3-dependent fetal hemoglobin production in human primary erythroid cells

Direct reprogramming of fibroblasts into neural stem cells by single non-neural progenitor transcription factor Ptf1a

Next‐generation disease modeling with direct conversion: a new path to old neurons

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