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Originally published In Press as doi:10.1074/mcp.M600443-MCP200 on February 22, 2007.
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Molecular & Cellular Proteomics 6:1007-1017, 2007.
© 2007 by The American Society for Biochemistry and Molecular Biology, Inc.


Research

Proteomics Analysis of Insulin Secretory Granules*,S

Yannick Brunner{ddagger}, Yohann Couté{ddagger}, Mariella Iezzi{ddagger}, Michelangelo Foti§, Mitsonuri Fukuda, Denis F. Hochstrasser{ddagger},||, Claes B. Wollheim§ and Jean-Charles Sanchez{ddagger},**

From the {ddagger} Biomedical Proteomics Research Group and § Department of Cell Physiology and Metabolism, University Medical Center, 1211 Geneva 4, Switzerland, Department of Developmental Biology and Neurosciences, Tohoku University, Sendai 980-8578 Japan, and || Central Clinical Chemistry Laboratory, Geneva University Hospital, 1211 Geneva 14, Switzerland

Insulin secretory granules (ISGs) are cytoplasmic organelles of pancreatic ß-cells. They are responsible for the storage and secretion of insulin. To date, only about 30 different proteins have been clearly described to be associated with these organelles. However, data from two-dimensional gel electrophoresis analyses suggested that almost 150 different polypeptides might be present within ISGs. The elucidation of the identity and function of the ISG proteins by proteomics strategies would be of considerable help to further understand some of the underlying mechanisms implicated in ISG biogenesis and trafficking. Furthermore it should give the bases to the comprehension of impaired insulin secretion observed during diabetes. A proteomics analysis of an enriched insulin granule fraction from the rat insulin-secreting cell line INS-1E was performed. The efficacy of the fractionation procedure was assessed by Western blot and electron microscopy. Proteins of the ISG fraction were separated by SDS-PAGE, excised from consecutive gel slices, and tryptically digested. Peptides were analyzed by nano-LC-ESI-MS/MS. This strategy identified 130 different proteins that were classified into four structural groups including intravesicular proteins, membrane proteins, novel proteins, and other proteins. Confocal microscopy analysis demonstrated the association of Rab37 and VAMP8 with ISGs in INS-1E cells. In conclusion, the present study identified 130 proteins from which 110 are new proteins associated with ISGs. The elucidation of their role will further help in the understanding of the mechanisms governing impaired insulin secretion during diabetes.


** To whom correspondence should be addressed: Biomedical Proteomics Research Group, DBSB/CMU, Rue Michel Servet 1, CH-1211 Genève 4, Switzerland. Tel.: 41-22-379-54-86; Fax: 41-22-379-59-84; E-mail: Jean-Charles.Sanchez{at}medecine.unige.ch


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