SLC30A3 Responds to Glucose- and Zinc Variations in ß-Cells and Is Critical for Insulin Production and In Vivo Glucose-Metabolism During ß-Cell Stress | Zendy

Kamille Smidt | Zendy; Niels Jessen | Zendy; Andreas Brønden Petersen | Zendy; Agnete Larsen | Zendy; Nils E. Magnusson | Zendy; Johanne Bruun Jeppesen | Zendy; Meredin Stoltenberg | Zendy; Janetta G. Culvenor | Zendy; Andrew Tsatsanis | Zendy; Birgitte Brock | Zendy; Ole Schmitz | Zendy; Lise Wogensen | Zendy; Ashley I. Bush | Zendy; Jørgen Rungby | Zendy

Open Access

SLC30A3 Responds to Glucose- and Zinc Variations in ß-Cells and Is Critical for Insulin Production and In Vivo Glucose-Metabolism During ß-Cell Stress

Author(s) -

Kamille Smidt,

Niels Jessen,

Andreas Brønden Petersen,

Agnete Larsen,

Nils E. Magnusson,

Johanne Bruun Jeppesen,

Meredin Stoltenberg,

Janetta G. Culvenor,

Andrew Tsatsanis,

Birgitte Brock,

Ole Schmitz,

Lise Wogensen,

Ashley I. Bush,

Jørgen Rungby

Publication year - 2009

Publication title -

plos one

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 0.99

H-Index - 332

ISSN - 1932-6203

DOI - 10.1371/journal.pone.0005684

Subject(s) - medicine , insulin , endocrinology , carbohydrate metabolism , streptozotocin , glucose transporter , secretion , biology , glucose uptake , cell culture , zinc , beta cell , chemistry , diabetes mellitus , islet , genetics , organic chemistry

Background Ion transporters of the Slc30A- (ZnT-) family regulate zinc fluxes into sub-cellular compartments. β-cells depend on zinc for both insulin crystallization and regulation of cell mass. Methodology/Principal Findings This study examined: the effect of glucose and zinc chelation on ZnT gene and protein levels and apoptosis in β-cells and pancreatic islets, the effects of ZnT-3 knock-down on insulin secretion in a β-cell line and ZnT-3 knock-out on glucose metabolism in mice during streptozotocin-induced β-cell stress. In INS-1E cells 2 mM glucose down-regulated ZnT-3 and up-regulated ZnT-5 expression relative to 5 mM. 16 mM glucose increased ZnT-3 and decreased ZnT-8 expression. Zinc chelation by DEDTC lowered INS-1E insulin content and insulin expression. Furthermore, zinc depletion increased ZnT-3- and decreased ZnT-8 gene expression whereas the amount of ZnT-3 protein in the cells was decreased. Zinc depletion and high glucose induced apoptosis and necrosis in INS-1E cells. The most responsive zinc transporter, ZnT-3, was investigated further; by immunohistochemistry and western blotting ZnT-3 was demonstrated in INS-1E cells. 44% knock-down of ZnT-3 by siRNA transfection in INS-1E cells decreased insulin expression and secretion. Streptozotocin-treated mice had higher glucose levels after ZnT-3 knock-out, particularly in overt diabetic animals. Conclusion/Significance Zinc transporting proteins in β-cells respond to variations in glucose and zinc levels. ZnT-3, which is pivotal in the development of cellular changes as also seen in type 2 diabetes (e.g. amyloidosis in Alzheimer's disease) but not previously described in β-cells, is present in this cell type, up-regulated by glucose in a concentration dependent manner and up-regulated by zinc depletion which by contrast decreased ZnT-3 protein levels. Knock-down of the ZnT-3 gene lowers insulin secretion in vitro and affects in vivo glucose metabolism after streptozotocin treatment.

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