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Co-culture with Mature Islet Cells Augments the Differentiation of Insulin-Producing Cells from Pluripotent Stem Cells

Authors
Oh, Bea JunOh, Seung-HoonChoi, Jin MyungJin, Sang-ManShim, Woo-YoungLee, Myung-ShikLee, Moon-KyuKim, Kwang-WonKim, Jae Hyeon
Issue Date
Feb-2015
Publisher
HUMANA PRESS INC
Keywords
Pluripotent stem cells; Insulin-producing cells; Co-culture; beta-cell differentiation; Diabetes; Transplantation
Citation
STEM CELL REVIEWS AND REPORTS, v.11, no.1, pp.62 - 74
Journal Title
STEM CELL REVIEWS AND REPORTS
Volume
11
Number
1
Start Page
62
End Page
74
URI
https://scholarworks.bwise.kr/gachon/handle/2020.sw.gachon/10832
DOI
10.1007/s12015-014-9554-8
ISSN
1550-8943
Abstract
Islet transplantation has been hampered by the shortage of islet donors available for diabetes therapy. However, pluripotent stem cells (PSCs) can be an alternative source of insulin-producing cells (IPCs) because of their capacity for self-renewal and differentiation. We described a method to efficiently differentiate PSCs into IPCs by co-culturing mature islets with directed-differentiated pancreatic endoderm (PE) cells from mouse and human PSCs. PE cells co-cultured with islet cells or islet cell-derived conditioned medium (CM) showed increased expression levels of beta-cell markers; significantly higher levels of proinsulin- and Newport Green (NG)-positive cells, which revealed the characteristics of insulin producing cells; and increased insulin secretion upon glucose stimulation. Co-culturing human PE cells with islet cells was also effective to differentiate PE cells into IPCs. Diabetic nude mice transplanted with co-cultured cells exhibited restored euglycemia, human C-peptide release, and improved glucose tolerance. Immunohistochemistry revealed that insulin+/C-peptide + cells existed in the grafted tissues. These results suggest that mature islet cells can increase the differentiation efficiency of PE cells into mature IPCs via paracrine effects.
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