Functional differentiation of human dental pulp stem cells into neuron-like cells exhibiting electrophysiological activity.

IF 7.3 2区医学 Q1 CELL & TISSUE ENGINEERING Stem Cell Research & Therapy Pub Date : 2025-01-23 DOI:10.1186/s13287-025-04134-7

B Pardo-Rodríguez, A M Baraibar, I Manero-Roig, J Luzuriaga, J Salvador-Moya, Y Polo, R Basanta-Torres, F Unda, S Mato, Gaskon Ibarretxe, Jose Ramon Pineda

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Abstract

Background and aim: Human dental pulp stem cells (hDPSCs) constitute a promising alternative for central nervous system (CNS) cell therapy. Unlike other human stem cells, hDPSCs can be differentiated, without genetic modification, to neural cells that secrete neuroprotective factors. However, a better understanding of their real capacity to give rise to functional neurons and integrate into synaptic networks is still needed. For that, ex vivo differentiation protocols must be refined, especially to avoid the use of fetal animal serum. The aim of our study is to improve existing differentiation protocols of hDPSCs into neuron-like cells.

Methods: We compared the effects of the (1) absence or presence of fetal serum during the initial expansion phase as a step prior to switching cultures to neurodifferentiation media. We (2) improved hDPSC neurodifferentiation by adding retinoic acid (RA) and potassium chloride (KCl) pulses for 21 or 60 days and characterized the results by immunofluorescence, digital morphometric analysis, RT-qPCR and electrophysiology.

Results: We found that neural markers like Nestin, GFAP, S100β and p75^NTR were expressed differently in neurodifferentiated hDPSC cultures depending on the presence or absence of serum during the initial cell expansion phase. In addition, hDPSCs previously grown as spheroids in serum-free medium exhibited in vitro expression of neuronal markers such as doublecortin (DCX), neuronal nuclear antigen (NeuN), Ankyrin-G and MAP2 after neurodifferentiation. Presynaptic vGLUT2, Synapsin-I, and excitatory glutamatergic and inhibitory GABAergic postsynaptic scaffold proteins and receptor subunits were also present in these neurodifferentiated hDPSCs. Treatment with KCl and RA increased the amount of both voltage-gated Na⁺ and K⁺ channel subunits in neurodifferentiated hDPSCs at the transcript level. Consistently, these cells displayed voltage-dependent K⁺ and TTX-sensitive Na⁺ currents as well as spontaneous electrophysiological activity and repetitive neuronal action potentials with a full baseline potential recovery.

Conclusion: Our study demonstrates that hDPSCs can be differentiated to neuronal-like cells that display functional excitability and thus evidence the potential of these easily accessible human stem cells for nerve tissue engineering. These results highlight the importance of choosing an appropriate culture protocol to successfully neurodifferentiate hDPSCs.

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人牙髓干细胞向具有电生理活性的神经元样细胞的功能分化。

背景与目的：人牙髓干细胞（hDPSCs）是一种很有前途的中枢神经系统（CNS）细胞治疗方法。与其他人类干细胞不同，hDPSCs可以不经过基因修饰而分化为分泌神经保护因子的神经细胞。然而，我们仍然需要更好地了解它们产生功能性神经元并整合到突触网络中的真正能力。为此，必须完善体外分化方案，特别是要避免使用胎动物血清。本研究的目的是改进现有的hdpsc向神经元样细胞的分化方案。方法：我们比较了(1)在初始扩张阶段胎儿血清缺失或存在的影响，作为将培养物转换为神经分化培养基之前的一步。我们(2)通过添加维甲酸（RA）和氯化钾（KCl）脉冲21或60天改善hDPSC神经分化，并通过免疫荧光、数字形态分析、RT-qPCR和电生理学对结果进行了表征。结果：我们发现神经标记物如Nestin、GFAP、S100β和p75NTR在神经分化的hDPSC培养物中表达不同，这取决于细胞初始扩增期是否存在血清。此外，先前在无血清培养基中培养成球形的hdpsc在体外神经分化后表现出双皮质素（DCX）、神经元核抗原（NeuN）、锚定蛋白g和MAP2等神经元标志物的表达。突触前vGLUT2、synapsin - 1、兴奋性谷氨酸能和抑制性gaba能突触后支架蛋白和受体亚基也存在于这些神经分化的hDPSCs中。KCl和RA在转录水平上增加了神经分化hDPSCs中电压门控Na+和K+通道亚基的数量。一致地，这些细胞表现出电压依赖性的K+和ttx敏感的Na+电流，以及自发的电生理活动和重复的神经元动作电位，并具有完全的基线电位恢复。结论：我们的研究表明，hDPSCs可以分化为具有功能性兴奋性的神经元样细胞，从而证明了这些易于获得的人类干细胞在神经组织工程中的潜力。这些结果强调了选择合适的培养方案对成功分化hdpsc的重要性。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Stem Cell Research & Therapy CELL BIOLOGY-MEDICINE, RESEARCH & EXPERIMENTAL

CiteScore

13.20

自引率

8.00%

发文量

525

审稿时长

1 months

期刊介绍： Stem Cell Research & Therapy serves as a leading platform for translational research in stem cell therapies. This international, peer-reviewed journal publishes high-quality open-access research articles, with a focus on basic, translational, and clinical research in stem cell therapeutics and regenerative therapies. Coverage includes animal models and clinical trials. Additionally, the journal offers reviews, viewpoints, commentaries, and reports.