SORCS1 is necessary for normal insulin secretory granule biogenesis in metabolically stressed β cells
Melkam A. Kebede, … , Anjon Audhya, Alan D. Attie
Melkam A. Kebede, … , Anjon Audhya, Alan D. Attie
Published October 1, 2014; First published August 26, 2014
Citation Information: J Clin Invest. 2014;124(10):4240-4256. https://doi.org/10.1172/JCI74072.
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Categories: Research Article Endocrinology

SORCS1 is necessary for normal insulin secretory granule biogenesis in metabolically stressed β cells

Abstract

We previously positionally cloned Sorcs1 as a diabetes quantitative trait locus. Sorcs1 belongs to the Vacuolar protein sorting-10 (Vps10) gene family. In yeast, Vps10 transports enzymes from the trans-Golgi network (TGN) to the vacuole. Whole-body Sorcs1 KO mice, when made obese with the leptinob mutation (ob/ob), developed diabetes. β Cells from these mice had a severe deficiency of secretory granules (SGs) and insulin. Interestingly, a single secretagogue challenge failed to consistently elicit an insulin secretory dysfunction. However, multiple challenges of the Sorcs1 KO ob/ob islets consistently revealed an insulin secretion defect. The luminal domain of SORCS1 (Lum-Sorcs1), when expressed in a β cell line, acted as a dominant-negative, leading to SG and insulin deficiency. Using syncollin-dsRed5TIMER adenovirus, we found that the loss of Sorcs1 function greatly impairs the rapid replenishment of SGs following secretagogue challenge. Chronic exposure of islets from lean Sorcs1 KO mice to high glucose and palmitate depleted insulin content and evoked an insulin secretion defect. Thus, in metabolically stressed mice, Sorcs1 is important for SG replenishment, and under chronic challenge by insulin secretagogues, loss of Sorcs1 leads to diabetes. Overexpression of full-length SORCS1 led to a 2-fold increase in SG content, suggesting that SORCS1 is sufficient to promote SG biogenesis.

Authors

Melkam A. Kebede, Angie T. Oler, Trillian Gregg, Allison J. Balloon, Adam Johnson, Kelly Mitok, Mary Rabaglia, Kathryn Schueler, Donald Stapleton, Candice Thorstenson, Lindsay Wrighton, Brendan J. Floyd, Oliver Richards, Summer Raines, Kevin Eliceiri, Nabil G. Seidah, Christopher Rhodes, Mark P. Keller, Joshua L. Coon, Anjon Audhya, Alan D. Attie

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Figure 3

Overexpressed Sorcs1a colocalizes with perinuclear Golgi stacks and some post-Golgi compartments.

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Overexpressed Sorcs1a colocalizes with perinuclear Golgi stacks and some...
Double staining with myc-Sorcs1 (red) and either the cis-Golgi matrix protein GM130 (A), the trans-Golgi protein TGN38 before (B) or after (C) brefeldin A treatment, the early endosomal protein Rab5 (D), or the SG marker chromogranin B (E) (green) of INS1 832/13 cells stably transfected with myc-tagged inducible Sorcs1a plasmid 18 hours after induction with 25 ng/ml doxycycline.