Human Pluripotent Stem Cell-Derived Neurons Are Functionally Mature In Vitro and Integrate into the Mouse Striatum Following Transplantation

被引:0
作者
Andrea Comella-Bolla
Javier G. Orlandi
Andrés Miguez
Marco Straccia
María García-Bravo
Georgina Bombau
Mireia Galofré
Phil Sanders
Jordi Carrere
José Carlos Segovia
Joan Blasi
Nicholas D. Allen
Jordi Alberch
Jordi Soriano
Josep M. Canals
机构
[1] University of Barcelona,Laboratory of Stem Cells and Regenerative Medicine, Department of Biomedicine, Faculty of Medicine and Health Science
[2] University of Barcelona,Production and validation center of advanced therapies (Creatio), Faculty of Medicine and Health Science
[3] University of Barcelona,Institute of Neurosciences
[4] Networked Biomedical Research Centre for Neurodegenerative Disorders,Pathophysiology of Neurodegenerative Disease. Laboratory, Department of Biomedicine, Faculty of Medicine and Health Science
[5] August Pi i Sunyer Biomedical Research Institute (IDIBAPS),Departament de Física de la Matèria Condensada
[6] University of Barcelona,Department of Physics and Astronomy
[7] University of Barcelona,Differentiation and Cytometry Unit, Division of Hematopoietic Innovative Therapies
[8] University of Calgary,Advanced Therapies Unit
[9] Centro de Investigaciones Energéticas Medioambientales y Tecnológicas and Centro de Investigación Biomédica en Red de Enfermedades Raras (CIEMAT/CIBERER),Laboratory of Cellular and Molecular Neurobiology, Department Pathology and Experimental Therapeutics,
[10] Instituto de Investigación Sanitaria Fundación Jiménez Díaz (IIS-FJD,Cardiff Repair Group, School of Biosciences and medicine
[11] UAM),Institute of Complex Systems (UBICS)
[12] University of Barcelona,undefined
[13] Cardiff University,undefined
[14] University of Barcelona,undefined
来源
Molecular Neurobiology | 2020年 / 57卷
关键词
Telencephalon; Neuronal differentiation; Striatum; Calcium imaging; Spike-inference analysis; Transplantation;
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学科分类号
摘要
Human pluripotent stem cells (hPSCs) are a powerful tool for modelling human development. In recent years, hPSCs have become central in cell-based therapies for neurodegenerative diseases given their potential to replace affected neurons. However, directing hPSCs into specific neuronal types is complex and requires an accurate protocol that mimics endogenous neuronal development. Here we describe step-by-step a fast feeder-free neuronal differentiation protocol to direct hPSCs to mature forebrain neurons in 37 days in vitro (DIV). The protocol is based upon a combination of specific morphogens, trophic and growth factors, ions, neurotransmitters and extracellular matrix elements. A human-induced PSC line (Ctr-Q33) and a human embryonic stem cell line (GEN-Q18) were used to reinforce the potential of the protocol. Neuronal activity was analysed by single-cell calcium imaging. At 8 DIV, we obtained a homogeneous population of hPSC-derived neuroectodermal progenitors which self-arranged in bi-dimensional neural tube-like structures. At 16 DIV, we generated hPSC-derived neural progenitor cells (NPCs) with mostly a subpallial identity along with a subpopulation of pallial NPCs. Terminal in vitro neuronal differentiation was confirmed by the expression of microtubule associated protein 2b (Map 2b) by almost 100% of hPSC-derived neurons and the expression of specific-striatal neuronal markers including GABA, CTIP2 and DARPP-32. HPSC-derived neurons showed mature and functional phenotypes as they expressed synaptic markers, voltage-gated ion channels and neurotransmitter receptors. Neurons displayed diverse spontaneous activity patterns that were classified into three major groups, namely “high”, “intermediate” and “low” firing neurons. Finally, transplantation experiments showed that the NPCs survived and differentiated within mouse striatum for at least 3 months. NPCs integrated host environmental cues and differentiated into striatal medium-sized spiny neurons (MSNs), which successfully integrated into the endogenous circuitry without teratoma formation. Altogether, these findings demonstrate the potential of this robust human neuronal differentiation protocol, which will bring new opportunities for the study of human neurodevelopment and neurodegeneration, and will open new avenues in cell-based therapies, pharmacological studies and alternative in vitro toxicology.
引用
收藏
页码:2766 / 2798
页数:32
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