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Effective Generation of Functional Pancreatic ß Cells from Human-Derived Dental Stem Cells of Apical Papilla and Bone-Marrow-Derived Stem Cells: A Comparative Study.
Abuarqoub, Duaa; Adwan, Sofia; Zaza, Rand; Wehaibi, Suha; Aslam, Nazneen; Jafar, Hanan; Qinnah, Nidal; Awidi, Abdalla.
Affiliation
  • Abuarqoub D; Department of Pharmacology and Biomedical Sciences, University of Petra, Amman 11196, Jordan.
  • Adwan S; Cell Therapy Center, The University of Jordan, Amman 11942, Jordan.
  • Zaza R; Department of Medical Laboratories, Faculty of Health Sciences, American University of Madaba, Madaba 11821, Jordan.
  • Wehaibi S; Cell Therapy Center, The University of Jordan, Amman 11942, Jordan.
  • Aslam N; Cell Therapy Center, The University of Jordan, Amman 11942, Jordan.
  • Jafar H; Cell Therapy Center, The University of Jordan, Amman 11942, Jordan.
  • Qinnah N; Cell Therapy Center, The University of Jordan, Amman 11942, Jordan.
  • Awidi A; School of Medicine, The University of Jordan, Amman 11942, Jordan.
Pharmaceuticals (Basel) ; 16(5)2023 Apr 26.
Article in En | MEDLINE | ID: mdl-37242432
Diabetes Mellitus Type 1 is an autoimmune disease that occurs due to the destruction of insulin-producing cells (ß cells), resulting in hyperglycemia. Therefore, diabetic patients depend on insulin treatment for the rest of their lives. Stem cells are considered a promising cellular therapy to replace the nonfunctional beta cells with functional and mature beta cells. Hence, in this study, we aimed to examine the potential of dental stem cells of apical papilla (SCAP) to differentiate into functional islet cell aggregates (ICAs), compared to the ICA generated from bone-marrow-derived stem cells (BM-MSCs). Our strategy was to induce the differentiation of SCAP and BM-MSCs into a definitive endoderm. The success of endodermal differentiation was determined by measuring the expression of definitive endodermal markers, FOXA2 and SOX-17, by flow cytometry. Next, the maturity and functionality of the differentiated cells were evaluated by measuring the amount of insulin and C-peptide secreted by the derived ICAs using ELISA. Additionally, the expression of mature beta cell markers-insulin, C-peptide, glucagon and PDX-1-was detected through confocal microscopy, while the staining of the mature islet-like clusters was detected by using diphenythiocarbazone (DTZ). Our results have shown that both SCAP and BM-MSCs were sequentially committed to a definitive pancreatic endoderm and ß-cell-like cells by upregulating the expression of FOXA2 and SOX17 significantly (**** p < 0.0000 and *** p = 0.0001), respectively. Moreover, the identity of ICAs was confirmed by DTZ-positive staining, as well as by the expression of C-peptide, Pdx-1, insulin and glucagon at day 14. It was noted that at day 14, differentiated ICAs released insulin and C-peptides in a significant manner (* p < 0.01, *** p = 0.0001), respectively, exhibiting in vitro functionality. Our results demonstrated for the first time that SCAP could be differentiated into pancreatic cell lineage in a similar manner to BM-MSCs, suggesting a new unambiguous and nonconventional source of stem cells that could be used for stem cell therapy to treat diabetes.
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Full text: 1 Collection: 01-internacional Database: MEDLINE Language: En Journal: Pharmaceuticals (Basel) Year: 2023 Document type: Article Affiliation country: Jordania Country of publication: Suiza

Full text: 1 Collection: 01-internacional Database: MEDLINE Language: En Journal: Pharmaceuticals (Basel) Year: 2023 Document type: Article Affiliation country: Jordania Country of publication: Suiza