Isolation and Culture of β-Like Cells From Porcine Wirsung Duct

Abstract We sought to develop a protocol to isolate and culture porcine Wirsung duct cells in order to determine their potency to differentiate into insulin-expressing β-like cells. The porcine Wirsung duct isolated by a surgical microdissection was digested with collagenase P and trypsin to dissoci...

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Veröffentlicht in:Transplantation proceedings 2009-05, Vol.41 (4), p.1363-1366
Hauptverfasser: Gioviale, M.C, Damiano, G, Montalto, G, Buscemi, G, Romano, M, Lo Monte, A.I
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Sprache:eng
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Zusammenfassung:Abstract We sought to develop a protocol to isolate and culture porcine Wirsung duct cells in order to determine their potency to differentiate into insulin-expressing β-like cells. The porcine Wirsung duct isolated by a surgical microdissection was digested with collagenase P and trypsin to dissociate ductal cells. These elements were cultured in serum-free supplemented media: for 2 weeks. Thereafter the cells were exposed to varying concentrations of glucose (0, 5.6, 17.8, and 25 mmol/L) to induce a β-like phenotype, as identified by immunohistochemical staining. Cell growth proceeded slowly for the first 2 weeks of culture. After glucose induction for 2 weeks, they formed pancreatic islet-like structures. These cells were stained for the pancreatic ductal cell marker cytokeratin-19 (CK-19) and the pancreatic endocrine markers insulin and glucagon. After the second week, 90% of cells were positive for CK-19. Up to 20.1% of the cells in pancreatic 3-dimensional structures induced by 17.8 mmol/L glucose were positive for insulin, and
ISSN:0041-1345
1873-2623
DOI:10.1016/j.transproceed.2009.02.062