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Dynamin 2 regulates biphasic insulin secretion and plasma glucose homeostasis
Fan Fan, … , Louis H. Philipson, Xuelin Lou
Fan Fan, … , Louis H. Philipson, Xuelin Lou
Published September 28, 2015
Citation Information: J Clin Invest. 2015;125(11):4026-4041. https://doi.org/10.1172/JCI80652.
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Research Article Endocrinology

Dynamin 2 regulates biphasic insulin secretion and plasma glucose homeostasis

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Abstract

Alterations in insulin granule exocytosis and endocytosis are paramount to pancreatic β cell dysfunction in diabetes mellitus. Here, using temporally controlled gene ablation specifically in β cells in mice, we identified an essential role of dynamin 2 GTPase in preserving normal biphasic insulin secretion and blood glucose homeostasis. Dynamin 2 deletion in β cells caused glucose intolerance and substantial reduction of the second phase of glucose-stimulated insulin secretion (GSIS); however, mutant β cells still maintained abundant insulin granules, with no signs of cell surface expansion. Compared with control β cells, real-time capacitance measurements demonstrated that exocytosis-endocytosis coupling was less efficient but not abolished; clathrin-mediated endocytosis (CME) was severely impaired at the step of membrane fission, which resulted in accumulation of clathrin-coated endocytic intermediates on the plasma membrane. Moreover, dynamin 2 ablation in β cells led to striking reorganization and enhancement of actin filaments, and insulin granule recruitment and mobilization were impaired at the later stage of GSIS. Together, our results demonstrate that dynamin 2 regulates insulin secretory capacity and dynamics in vivo through a mechanism depending on CME and F-actin remodeling. Moreover, this study indicates a potential pathophysiological link between endocytosis and diabetes mellitus.

Authors

Fan Fan, Chen Ji, Yumei Wu, Shawn M. Ferguson, Natalia Tamarina, Louis H. Philipson, Xuelin Lou

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Figure 4

Dnm2 KO β cells maintain normal Ca2+ signaling and glucose metabolism.

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Dnm2 KO β cells maintain normal Ca2+ signaling and glucose metabolism.
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(A) Transmission and fluorescence images of islets after fura-2 AM loading. Scale bar: 50 μm. (B) Representative cytosolic Ca2+ ([Ca2+]i) dynamics in response to 12.8 mM glucose and 30 mM KCl. (C) Average [Ca2+]i amplitude changes (n = 15 islets for each group; 2-tailed t test). (D) Representative Ca2+ current, (E) Cm, and (F) average amplitude and density of Ca2+ current (n = 14 and 15 cells for control and Dnm2 KO cells, respectively). (G) Excitation spectrum of NADPH fluorescence in islets and (H) the fluorescence increase induced by 20 mM glucose in individual islets. (I) Average NADPH signal at rest and during 20 mM glucose stimulation (n = 15 islets in control; n = 13 in Dnm2 KO). *P < 0.05.

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