Imaging analysis reveals mechanistic differences between first- and second-phase insulin exocytosis

Author:

Ohara-Imaizumi Mica1,Fujiwara Tomonori2,Nakamichi Yoko1,Okamura Tadashi3,Akimoto Yoshihiro4,Kawai Junko15,Matsushima Satsuki6,Kawakami Hayato4,Watanabe Takashi6,Akagawa Kimio2,Nagamatsu Shinya1

Affiliation:

1. Department of Biochemistry

2. Department of Cell Physiology

3. Division of Animal Models, Department of Infectious Diseases, Research Institute, International Medical Center of Japan, Tokyo 162-8655, Japan

4. Department of Anatomy,

5. Department of Medicine, Metabolism and Endocrinology, Juntendo University School of Medicine, Tokyo, 113-8421, Japan

6. Department of Clinical Pathology, Kyorin University School of Medicine, Mitaka, Tokyo 181-8611, Japan

Abstract

The mechanism of glucose-induced biphasic insulin release is unknown. We used total internal reflection fluorescence (TIRF) imaging analysis to reveal the process of first- and second-phase insulin exocytosis in pancreatic β cells. This analysis showed that previously docked insulin granules fused at the site of syntaxin (Synt)1A clusters during the first phase; however, the newcomers fused during the second phase external to the Synt1A clusters. To reveal the function of Synt1A in phasic insulin exocytosis, we generated Synt1A-knockout (Synt1A−/−) mice. Synt1A−/− β cells showed fewer previously docked granules with no fusion during the first phase; second-phase fusion from newcomers was preserved. Rescue experiments restoring Synt1A expression demonstrated restoration of granule docking status and fusion events. Inhibition of other syntaxins, Synt3 and Synt4, did not affect second-phase insulin exocytosis. We conclude that the first phase is Synt1A dependent but the second phase is not. This indicates that the two phases of insulin exocytosis differ spatially and mechanistically.

Publisher

Rockefeller University Press

Subject

Cell Biology

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