Postdoctoral research fellow
Cellular & Physiological Sciences
The University of British Columbia
A Strategy to Differentiate Human Pluripotent Stem Cells into Insulin-producing Islet Clusters
Shenghui Liang1, Jia Zhao1, Mitchell Braam1, Robert Baker1, Priye Iworima1, Nina Quiskamp2, Timothy Kieffer1.
1Cellular & Physiological Sciences, The University of British Columbia, Vancouver, BC, Canada; 2STEMCELL Technologies, Vanoucer, BC, Canada
Introduction: While excellent glycemic control without insulin injections can be achieved by transplantation of cadaveric islets, this strategy is severely limited by donor availability thus hampering its broader application to diabetes treatment. Differentiation of human pluripotent stem cells (hPSCs) to insulin-secreting beta cells offers an alternative, unlimited source of transplantable material. However, stem cell-derived beta cells made using current approaches typically remain functionally immature and do not fully resemble bona fide natural beta cells.
Method: Building upon our previous studies in developing methods of generating islet cells from hPSCs, in this work we employed a hybrid strategy – combination of the STEMdiffTM Pancreatic Progenitor Kit (from stage 1-4) and a modified Rezania’s 2014 Nature Biotechnology method (termed as “R-protocol” hereafter from stage 5-7) – in order to further improve the differentiation consistency and outcomes.
Results: With the STEMdiffTM Pancreatic Progenitor Kit, we consistently differentiated Mel1 INSGFP/W hESCs (an insulin reporter line) into pancreatic progenitors in which over 80% of cells co-express key markers PDX1 and NKX6.1. Following the planar culture from stage 1-4, we used AggreWellTM plates to generate pancreatic progenitor clusters with uniform size and morphology. With modifications, we used R-protocol to further differentiate pancreatic progenitors into islet clusters and switched the cultures to a static suspension format for endocrine differentiation. At the end of differentiation, flow cytometry and immunostaining analysis showed that these islet clusters were comprised of three major islet cell types including insulin-expressing beta cells, glucagon-expressing alpha cells and somatostatin-expressing delta cells, as well as expressed transcription factors key in beta cell maturation. In vitro functional assessment further showed that the islet clusters displayed dynamic insulin secretion in response to glucose and an incretin hormone as well as depolarization challenge, yet did not fully mimic primary human islets.
Conclusion: Future efforts will focus on continued optimization of the differentiation protocols and increasing the scale to manufacture more mature islet cells, demonstrating applications of these stem cell-derived islet clusters in disease modeling, drug screening, and ultimately diabetes reversal.
Michael Smith Health Research BC. JDRF. CIHR.
References:
[1] Rezania, A., Bruin, J.E., Arora, P., Rubin, A., Batushansky, I., Asadi, A., O'Dwyer, S., Quiskamp, N., Mojibian,
M., Albrecht, T., et al. (2014). Reversal of diabetes with insulin-producing cells derived in vitro from human
pluripotent stem cells. Nat Biotechnol 32, 1121-1133. 10.1038/nbt.3033.
[2] Pagliuca, F.W., Millman, J.R., Gurtler, M., Segel, M., Van Dervort, A., Ryu, J.H., Peterson, Q.P., Greiner, D.,
and Melton, D.A. (2014). Generation of functional human pancreatic beta cells in vitro. Cell 159, 428-439.
10.1016/j.cell.2014.09.040.
[3] Balboa, D., Barsby, T., Lithovius, V., Saarimaki-Vire, J., Omar-Hmeadi, M., Dyachok, O., Montaser, H., Lund,
P.E., Yang, M., Ibrahim, H., et al. (2022). Functional, metabolic and transcriptional maturation of human
pancreatic islets derived from stem cells. Nat Biotechnol 40, 1042-1055. 10.1038/s41587-022-01219-z.
Lectures by Shenghui Liang
| When | Session | Talk Title | Room |
|---|---|---|---|
|
Mon-24 00:00 - 00:00 |
Video Posters - Will be available starting the week before the Summit |
A strategy to differentiate human pluripotent stem cells into insulin-producing islet clusters |