4.5 Article

Insulin action on protein synthesis and its association with eIF5A expression and hypusination

Journal

MOLECULAR BIOLOGY REPORTS
Volume 46, Issue 1, Pages 587-596

Publisher

SPRINGER
DOI: 10.1007/s11033-018-4512-1

Keywords

Myoblast cells; Insulin; Protein synthesis; eIF5A; Hypusine

Funding

  1. Sao Paulo Research Foundation (FAPESP) [2010/18095-0]
  2. FAPESP [2013/20504-3, 2013/23620-4, 2014/27154-0, 2017/21914-1]

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The hormone insulin plays a central role in the metabolism of carbohydrates, lipids, and proteins. In relation to protein metabolism, insulin stimulates amino acid uptake and activates protein synthesis in responsive cells by modulation of signal transduction pathways, such as associated to Akt/PkB, mTOR, S6Ks, 4E-BP1, and several translation initiation/elongation factors. In this context, there is no information on direct cellular treatment with insulin and effects on eukaryotic translation initiation factor 5A (eIF5A) regulation. The eIF5A protein contains an exclusive amino acid residue denominated hypusine, which is essential for its activity and synthesized by posttranslational modification of a specific lysine residue using spermidine as substrate. The eIF5A protein is involved in cellular proliferation and differentiation processes, as observed for satellite cells derived from rat muscles, revealing that eIF5A has an important role in muscle regeneration. The aim of this study was to determine whether eIF5A expression and hypusination are influenced by direct treatment of insulin on L6 myoblast cells. We observed that insulin increased the content of eIF5A transcripts. This effect occurred in cells treated or depleted of fetal bovine serum, revealing a positive insulin effect independent of other serum components. In addition, it was observed that hypusination follows the maintenance of eIF5A protein content in the serum depleted cells and treated with insulin. These results demonstrate that eIF5A is modulated by insulin, contributing the protein synthesis machinery control, as observed by puromycin incorporation in nascent proteins.

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