2. Academic Validation
  3. An integrin binding-defective mutant of insulin-like growth factor-1 (R36E/R37E IGF1) acts as a dominant-negative antagonist of the IGF1 receptor (IGF1R) and suppresses tumorigenesis but still binds to IGF1R

An integrin binding-defective mutant of insulin-like growth factor-1 (R36E/R37E IGF1) acts as a dominant-negative antagonist of the IGF1 receptor (IGF1R) and suppresses tumorigenesis but still binds to IGF1R

  • J Biol Chem. 2013 Jul 5;288(27):19593-603. doi: 10.1074/jbc.M113.470872.
Masaaki Fujita 1 Katsuaki Ieguchi Dora M Cedano-Prieto Andrew Fong Charles Wilkerson Jane Q Chen Mac Wu Su-Hao Lo Anthony T W Cheung Machelle D Wilson Robert D Cardiff Alexander D Borowsky Yoko K Takada Yoshikazu Takada
Affiliations

Affiliation

  • 1 Department of Dermatology, University of California Davis School of Medicine, Sacramento, California 95817, USA.
PMID: 23696648 DOI: 10.1074/jbc.M113.470872
Abstract

Insulin-like growth factor-1 (IGF1) is a major therapeutic target for Cancer. We recently reported that IGF1 directly binds to integrins (αvβ3 and α6β4) and induces ternary complex formation (integrin-IGF1-IGF1 receptor (IGF1R)) and that the Integrin binding-defective mutant of IGF1 (R36E/R37E) is defective in signaling and ternary complex formation. These findings predict that R36E/R37E competes with WT IGF1 for binding to IGF1R and inhibits IGF signaling. Here, we described that excess R36E/R37E suppressed cell viability increased by WT IGF1 in vitro in non-transformed cells. We studied the effect of R36E/R37E on viability and tumorigenesis in Cancer cell lines. We did not detect an effect of WT IGF1 or R36E/R37E in Cancer cells under anchorage-dependent conditions. However, under anchorage-independent conditions, WT IGF1 enhanced cell viability and induced signals, whereas R36E/R37E did not. Notably, excess R36E/R37E suppressed cell viability and signaling induced by WT IGF1 under anchorage-independent conditions. Using Cancer cells stably expressing WT IGF1 or R36E/R37E, we determined that R36E/R37E suppressed tumorigenesis in vivo, whereas WT IGF1 markedly enhanced it. R36E/R37E suppressed the binding of WT IGF1 to the cell surface and the subsequent ternary complex formation induced by WT IGF1. R36E/R37E suppressed activation of IGF1R by Insulin. WT IGF1, but not R36E/R37E, induced ternary complex formation with the IGF1R/Insulin Receptor hybrid. These findings suggest that 1) IGF1 induces signals under anchorage-independent conditions and that 2) R36E/R37E acts as a dominant-negative inhibitor of IGF1R (IGF1 decoy). Our results are consistent with a model in which ternary complex formation is critical for IGF signaling.

Keywords

Cancer; Drug Discovery; Extracellular Matrix; Growth Factors; Insulin-like Growth Factor (IGF); Integrins; Mutant; Signal Transduction.

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