Regulation of multiple signaling pathways promotes the consistent expansion of human pancreatic progenitors in defined conditions

Author:

Jarc Luka,Bandral Manuj,Zanfrini Elisa,Lesche Mathias,Kufrin Vida,Sendra Raquel,Pezzolla Daniela,Giannios Ioannis,Khattak Shahryar,Neumann Katrin,Ludwig Barbara,Gavalas Anthony

Abstract

ABSTRACTThe unlimited expansion of human progenitor cells in vitro could unlock many prospects for regenerative medicine. However, it remains an important challenge as it requires the decoupling of the mechanisms supporting progenitor self-renewal and expansion from those mechanisms promoting their differentiation. This study focuses on the expansion of human pluripotent stem (hPS) cell derived pancreatic progenitors (PP) to advance novel therapies for diabetes.We obtained mechanistic insights into PP expansion requirements and, through a hypothesis-driven iterative approach, identified conditions for the robust and unlimited expansion of hPS cell derived PP cells under GMP-compliant conditions. We show that the combined stimulation of specific mitogenic pathways, suppression of retinoic acid signaling and inhibition of selected branches of the TGFβ and Wnt signaling pathways are necessary for the effective decoupling of PP proliferation from differentiation. This enabled the reproducible, 2000-fold, over ten passages and 40-45 days, expansion of PDX1+/SOX9+/NKX6-1+PP cells. Transcriptome analyses confirmed the stabilisation of PP identity and the effective suppression of differentiation. Using these conditions, PDX1+/SOX9+/NKX6-1+PP cells, derived from different, both XY and XX, hPS cells lines, were enriched to nearly 90% homogeneity and expanded with very similar kinetics and efficiency. Furthermore, non-expanded and expanded PP cells, from different hPS cell lines, were differentiated in microwells into homogeneous islet-like clusters (SC-islets) with very similar efficiency. These clusters contained abundant β-cells of comparable functionality as assessed by glucose-stimulated insulin secretion assays.These findings established the signaling requirements to decouple PP proliferation from differentiation and allowed the consistent expansion of hPS cell derived PP cells. They will enable the establishment of large banks of GMP-derived PP cells derived from diverse hPS cell lines. This approach will streamline SC-islet production for further development of the differentiation process, diabetes research, personalized medicine and cell therapies.

Publisher

Cold Spring Harbor Laboratory

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