Self-organized insulin-producing β-cells differentiated from human omentum-derived stem cells and their in vivo therapeutic potential

Authors
Jeong, Ji HoonPark, Ki NamKim, Joo HyunNoh, KyungmuHur, Sung SikKim, YunhyeHong, MoonjuChung, Jun ChulPark, Jae HongLee, JongsoonSon, Young-IkLee, Ju HunKim, Sang-HeonHwang, Yongsung
Issue Date
2023-08
Publisher
The Korean Society for Biomaterials | BioMed Central
Citation
Biomaterials Research, v.27, no.1, pp.1999 - 2016
Abstract
Background Human omentum-derived mesenchymal stem cells (hO-MSCs) possess great potential to differentiate into multiple lineages and have self-renewal capacity, allowing them to be utilized as patient-specific cell-based therapeutics. Although the use of various stem cell-derived ss-cells has been proposed as a novel approach for treating diabetes mellitus, developing an efficient method to establish highly functional ss-cells remains challenging. Methods We aimed to develop a novel cell culture platform that utilizes a fibroblast growth factor 2 (FGF2)-immobilized matrix to regulate the adhesion and differentiation of hO-MSCs into insulin-producing ss-cells via cell-matrix/ cell-cell interactions. In our study, we evaluated the in vitro differentiation potential of hO-MSCs cultured on an FGF2immobilized matrix and a round-bottom plate (RBP). Further, the in vivo therapeutic efficacy of the ss-cells transplanted into kidney capsules was evaluated using animal models with streptozotocin (STZ)-induced diabetes. Results Our findings demonstrated that cells cultured on an FGF2-immobilized matrix could self-organize into insulin-producing ss-cell progenitors, as evident from the upregulation of pancreatic ss-cell-specific markers (PDX-1, Insulin, and Glut-2). Moreover, we observed significant upregulation of heparan sulfate proteoglycan, gap junction proteins (Cx36 and Cx43), and cell adhesion molecules (E-cadherin and Ncam1) in cells cultured on the FGF2-immobilized matrix. In addition, in vivo transplantation of differentiated ss-cells into animal models of STZ-induced diabetes revealed their survival and engraftment as well as glucose-sensitive production of insulin within the host microenvironment, at over 4 weeks after transplantation. Conclusions Our findings suggest that the FGF2-immobilized matrix can support initial cell adhesion, maturation, and glucose-stimulated insulin secretion within the host microenvironment. Such a cell culture platform can offer novel strategies to obtain functional pancreatic ss- cells from patient-specific cell sources, ultimately enabling better treatment for diabetes mellitus.
Keywords
MOLECULE N-CAM; STROMAL CELLS; EXTRACELLULAR-MATRIX; PANCREATIC-ISLETS; ADHESION; EXPRESSION; CALCIUM; CLUSTER; SCAFFOLD; MARROW; Pancreatic beta-cells; Cell adhesion; Insulin-producing cells; Cell-to-cell interaction; Fibroblast growth factor 2; Stem cell differentiation; Streptozotocin-induced diabetic models
ISSN
1226-4601
URI
https://pubs.kist.re.kr/handle/201004/113385
DOI
10.1186/s40824-023-00419-1
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KIST Article > 2023
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