Literature DB >> 19183938

Differentiation of COPAS-sorted non-endocrine pancreatic cells into insulin-positive cells in the mouse.

R Kikugawa1, H Katsuta, T Akashi, S Yatoh, G C Weir, A Sharma, S Bonner-Weir.   

Abstract

AIMS/HYPOTHESIS: The regenerative process in the pancreas is of particular interest, since insulin-producing beta cells are lost in diabetes. Differentiation of new beta cells from pancreatic non-endocrine cells has been reported in vivo and in vitro, a finding that implies the existence of pancreatic stem/progenitor cells. However, while tissue-specific stem cells are well documented in skin, intestine and testis, pancreatic stem cells have been elusive. We hypothesised that pancreatic stem/progenitor cells within the non-endocrine fraction could be a source of new islets in vitro.
METHODS: To test if there were such cells within the pancreas, we generated pancreatic cell aggregates from tissue remaining after islet isolation from mouse insulin promoter 1-green fluorescent protein (MIP-GFP) mice. To eliminate any contamination of insulin-positive cells, we deleted all GFP-positive aggregates using COPAS Select and cultured with Matrigel. Immunohistochemistry, quantitative real-time PCR and single-cell nested RT-PCR were performed to confirm formation of insulin-producing cells.
RESULTS: The GFP-negative cells were expanded as monolayers and then differentiated into three-dimensional cystic structures. After 1 week of culture, GFP-positive cells were found as clusters or single cells. By quantitative real-time PCR, no insulin mRNA was detected immediately after COPAS sorting, but after differentiation insulin mRNA of the whole preparation was 1.91 +/- 0.31% that of purified MIP-GFP beta cells. All GFP-positive cells expressed insulin 1; most expressed insulin 2, pancreas duodenum homeobox-1 and cytokeratin 19 by single cell nested RT-PCR. CONCLUSIONS/
INTERPRETATION: Our data support the concept that within the exocrine (acinar and ductal) pancreas of the adult mouse there are cells that can give rise to insulin-positive cells in vitro.

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Year:  2009        PMID: 19183938      PMCID: PMC4336153          DOI: 10.1007/s00125-009-1260-8

Source DB:  PubMed          Journal:  Diabetologia        ISSN: 0012-186X            Impact factor:   10.122


  33 in total

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2.  Validation of large particle flow cytometry for the analysis and sorting of intact pancreatic islets.

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3.  Isolation of mouse pancreatic ductal progenitor cells expressing CD133 and c-Met by flow cytometric cell sorting.

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5.  In vitro neogenesis of human islets reflects the plasticity of differentiated human pancreatic cells.

Authors:  R Gao; J Ustinov; O Korsgren; T Otonkoski
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6.  In vitro cultivation of human islets from expanded ductal tissue.

Authors:  S Bonner-Weir; M Taneja; G C Weir; K Tatarkiewicz; K H Song; A Sharma; J J O'Neil
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1.  Complete disassociation of adult pancreas into viable single cells through cold trypsin-EDTA digestion.

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Review 2.  Stem cell therapy for type 1 diabetes mellitus.

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Journal:  Nat Rev Endocrinol       Date:  2010-03       Impact factor: 43.330

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Review 5.  Pancreatic stem/progenitor cells for the treatment of diabetes.

Authors:  Hirofumi Noguchi
Journal:  Rev Diabet Stud       Date:  2010-08-10

Review 6.  β-cell replacement sources for type 1 diabetes: a focus on pancreatic ductal cells.

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7.  Intraislet Pancreatic Ducts Can Give Rise to Insulin-Positive Cells.

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8.  Purified human pancreatic duct cell culture conditions defined by serum-free high-content growth factor screening.

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9.  FGF-2b and h-PL Transform Duct and Non-Endocrine Human Pancreatic Cells into Endocrine Insulin Secreting Cells by Modulating Differentiating Genes.

Authors:  Giulia Donadel; Donatella Pastore; David Della-Morte; Barbara Capuani; Marco F Lombardo; Francesca Pacifici; Marco Bugliani; Fabio A Grieco; Piero Marchetti; Davide Lauro
Journal:  Int J Mol Sci       Date:  2017-10-25       Impact factor: 5.923

  9 in total

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