Literature DB >> 29139614

Human dental stem cell derived transgene-free iPSCs generate functional neurons via embryoid body-mediated and direct induction methods.

Ikbale El Ayachi1, Jun Zhang1, Xiao-Ying Zou2, Dong Li1, Zongdong Yu1, Wei Wei3, Kristen M S O'Connell3, George T-J Huang1,2.   

Abstract

Induced pluripotent stem cells (iPSCs) give rise to neural stem/progenitor cells, serving as a good source for neural regeneration. Here, we established transgene-free (TF) iPSCs from dental stem cells (DSCs) and determined their capacity to differentiate into functional neurons in vitro. Generated TF iPSCs from stem cells of apical papilla and dental pulp stem cells underwent two methods-embryoid body-mediated and direct induction, to guide TF-DSC iPSCs along with H9 or H9 Syn-GFP (human embryonic stem cells) into functional neurons in vitro. Using the embryoid body-mediated method, early stage neural markers PAX6, SOX1, and nestin were detected by immunocytofluorescence or reverse transcription-real time polymerase chain reaction (RT-qPCR). At late stage of neural induction measured at Weeks 7 and 9, the expression levels of neuron-specific markers Nav1.6, Kv1.4, Kv4.2, synapsin, SNAP25, PSD95, GAD67, GAP43, and NSE varied between stem cells of apical papilla iPSCs and H9. For direct induction method, iPSCs were directly induced into neural stem/progenitor cells and guided to become neuron-like cells. The direct method, while simpler, showed cell detachment and death during the differentiation process. At early stage, PAX6, SOX1 and nestin were detected. At late stage of differentiation, all five genes tested, nestin, βIII-tubulin, neurofilament medium chain, GFAP, and Nav, were positive in many cells in cultures. Both differentiation methods led to neuron-like cells in cultures exhibiting sodium and potassium currents, action potential, or spontaneous excitatory postsynaptic potential. Thus, TF-DSC iPSCs are capable of undergoing guided neurogenic differentiation into functional neurons in vitro, thereby may serve as a cell source for neural regeneration.
Copyright © 2017 John Wiley & Sons, Ltd.

Entities:  

Keywords:  DPSCs; DSCs; ESCs; SCAP; adult stem cells; dental stem cells; electrophysiology; embryonic stem cells; iPSCs; in vitro; induced pluripotent stem cells; neurogenesis; patch clamp; reprogramming; transgene-free

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Substances:

Year:  2018        PMID: 29139614      PMCID: PMC6482049          DOI: 10.1002/term.2615

Source DB:  PubMed          Journal:  J Tissue Eng Regen Med        ISSN: 1932-6254            Impact factor:   3.963


  62 in total

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Authors:  Zongdong Yu; Philippe Gauthier; Quynh T Tran; Ikbale El-Ayachi; Fazal-Ur-Rehman Bhatti; Rayan Bahabri; Mey Al-Habib; George Tj Huang
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  6 in total

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Review 2.  Neuro-regenerative potential of dental stem cells: a concise review.

Authors:  Duaa Abuarqoub; Nazneen Aslam; Bayan Almajali; Leen Shajrawi; Hanan Jafar; Abdalla Awidi
Journal:  Cell Tissue Res       Date:  2020-07-28       Impact factor: 5.249

3.  Human Dental Pulp Stem Cells and Gingival Mesenchymal Stem Cells Display Action Potential Capacity In Vitro after Neuronogenic Differentiation.

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Journal:  Stem Cell Rev Rep       Date:  2019-02       Impact factor: 5.739

4.  Potential of tailored amorphous multiporous calcium silicate glass for pulp capping regenerative endodontics-A preliminary assessment.

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Journal:  Front Genet       Date:  2018-10-08       Impact factor: 4.599

6.  Isolation and culture of dental pulp stem cells from permanent and deciduous teeth.

Authors:  Shagufta Naz; Farhan Raza Khan; Raheela Rahmat Zohra; Sahreena Salim Lakhundi; Mehwish Sagheer Khan; Nuruddin Mohammed; Tashfeen Ahmad
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  6 in total

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