Pronounced proliferation of non-beta cells in response to beta-cell mitogens in isolated human islets of Langerhans

Author:

Maachi Hasna,Ghislain Julien,Tremblay Caroline,Poitout Vincent

Abstract

AbstractThe potential to treat diabetes by increasing beta-cell mass is driving a major effort to identify beta-cell mitogens. Demonstration of mitogen activity in human beta cells is frequently performed in ex vivo assays. However, reported disparities in the efficacy of beta-cell mitogens led us to investigate the sources of this variability. We studied 35 male (23) and female (12) human islet batches covering a range of donor ages and BMI. Islets were kept intact or dispersed into single cells and cultured in the presence of harmine, glucose, or heparin-binding epidermal growth factor-like growth factor (HB-EGF), and subsequently analyzed by immunohistochemistry or flow cytometry. Proliferating cells were identified by double labeling with EdU and Ki67 and glucagon, c-peptide or Nkx6.1, and cytokeratin-19 to respectively label alpha, beta, and ductal cells. Harmine and HB-EGF stimulated human beta-cell proliferation, but the effect of glucose was dependent on the assay and the donor. Harmine potently stimulated alpha-cell proliferation and both harmine and HB-EGF increased proliferation of insulin- and glucagon-negative cells, including cytokeratin 19-positive cells. Given the abundance of non-beta cells in human islet preparations, our results suggest that assessment of beta-cell mitogens requires complementary approaches and rigorous identification of cell identity using multiple markers.

Funder

Fonds de Recherche du Québec - Santé

National Institute of Diabetes and Digestive and Kidney Diseases

Canadian Institutes of Health Research

Quebec Cardiometabolic Health, Diabetes and Obesity Research Network

Integrated Islet Distribution Program

Publisher

Springer Science and Business Media LLC

Subject

Multidisciplinary

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