Propensity of Patient-Derived iPSCs for Retinal Differentiation: Implications for Autologous Cell Replacement

诱导多能干细胞 视网膜 计算生物学 生物 医学 眼科 生物信息学 遗传学 基因 胚胎干细胞
作者
Jessica A. Cooke,Andrew P. Voigt,Michael A. Collingwood,Nicholas Stone,S. Scott Whitmore,Adam P. DeLuca,Erin R. Burnight,Kristin R. Anfinson,Christopher A. Vakulskas,Austin J Reutzel,Heather T. Daggett,Jeaneen L. Andorf,Edwin M. Stone,Robert F. Mullins,Budd A. Tucker
出处
期刊:Stem Cells Translational Medicine [Wiley]
卷期号:12 (6): 365-378 被引量:10
标识
DOI:10.1093/stcltm/szad028
摘要

Prior to use, newly generated induced pluripotent stem cells (iPSC) should be thoroughly validated. While excellent validation and release testing assays designed to evaluate potency, genetic integrity, and sterility exist, they do not have the ability to predict cell type-specific differentiation capacity. Selection of iPSC lines that have limited capacity to produce high-quality transplantable cells, places significant strain on valuable clinical manufacturing resources. The purpose of this study was to determine the degree and root cause of variability in retinal differentiation capacity between cGMP-derived patient iPSC lines. In turn, our goal was to develop a release testing assay that could be used to augment the widely used ScoreCard panel. IPSCs were generated from 15 patients (14-76 years old), differentiated into retinal organoids, and scored based on their retinal differentiation capacity. Despite significant differences in retinal differentiation propensity, RNA-sequencing revealed remarkable similarity between patient-derived iPSC lines prior to differentiation. At 7 days of differentiation, significant differences in gene expression could be detected. Ingenuity pathway analysis revealed perturbations in pathways associated with pluripotency and early cell fate commitment. For example, good and poor producers had noticeably different expressions of OCT4 and SOX2 effector genes. QPCR assays targeting genes identified via RNA sequencing were developed and validated in a masked fashion using iPSCs from 8 independent patients. A subset of 14 genes, which include the retinal cell fate markers RAX, LHX2, VSX2, and SIX6 (all elevated in the good producers), were found to be predictive of retinal differentiation propensity.

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