The use of a SOX10 reporter toward ameliorating oligodendrocyte lineage differentiation from human induced pluripotent stem cells

Author:

Piscopo Valerio E. C.12ORCID,Chapleau Alexandra123ORCID,Blaszczyk Gabriela J.124ORCID,Sirois Julien12ORCID,You Zhipeng12,Soubannier Vincent12ORCID,Chen Carol X.‐Q.12ORCID,Bernard Geneviève2356ORCID,Antel Jack P.24ORCID,Durcan Thomas M.12ORCID

Affiliation:

1. Early Drug Discovery Unit, Montreal Neurological Institute‐Hospital McGill University Montreal Quebec Canada

2. Department of Neurology and Neurosurgery McGill University Montreal Quebec Canada

3. Child Health and Human Development Program Research Institute of the McGill University Health Center Montreal Quebec Canada

4. Neuroimmunology Unit, Montreal Neurological Institute‐Hospital McGill University Montreal Quebec Canada

5. Department of Pediatrics and Human Genetics McGill University Montreal Quebec Canada

6. Division of Medical Genetics, Department of Internal Medicine McGill University Health Center Montreal Quebec Canada

Abstract

AbstractOligodendrocytes (OLs) are key players in the central nervous system, critical for the formation and maintenance of the myelin sheaths insulating axons, ensuring efficient neuronal communication. In the last decade, the use of human induced pluripotent stem cells (iPSCs) has become essential for recapitulating and understanding the differentiation and role of OLs in vitro. Current methods include overexpression of transcription factors for rapid OL generation, neglecting the complexity of OL lineage development. Alternatively, growth factor‐based protocols offer physiological relevance but struggle with efficiency and cell heterogeneity. To address these issues, we created a novel SOX10‐P2A‐mOrange iPSC reporter line to track and purify oligodendrocyte precursor cells. Using this reporter cell line, we analyzed an existing differentiation protocol and shed light on the origin of glial cell heterogeneity. Additionally, we have modified the differentiation protocol, toward enhancing reproducibility, efficiency, and terminal maturity. Our approach not only advances OL biology but also holds promise to accelerate research and translational work with iPSC‐derived OLs.

Funder

Canada First Research Excellence Fund

Fonds de Recherche du Québec - Santé

Canadian Institutes of Health Research

Fondation du Grand défi Pierre Lavoie

Publisher

Wiley

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