Increased sugar uptake promotes oncogenesis via EPAC/RAP1 and O-GlcNAc pathways
Yasuhito Onodera, … , Jin-Min Nam, Mina J. Bissell
Yasuhito Onodera, … , Jin-Min Nam, Mina J. Bissell
Published December 9, 2013
Citation Information: J Clin Invest. 2014;124(1):367-384. https://doi.org/10.1172/JCI63146.
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Research Article Oncology

Increased sugar uptake promotes oncogenesis via EPAC/RAP1 and O-GlcNAc pathways

Abstract

There is a considerable resurgence of interest in the role of aerobic glycolysis in cancer; however, increased glycolysis is frequently viewed as a consequence of oncogenic events that drive malignant cell growth and survival. Here we provide evidence that increased glycolytic activation itself can be an oncogenic event in a physiologically relevant 3D culture model. Overexpression of glucose transporter type 3 (GLUT3) in nonmalignant human breast cells activated known oncogenic signaling pathways, including EGFR, β1 integrin, MEK, and AKT, leading to loss of tissue polarity and increased growth. Conversely, reduction of glucose uptake in malignant cells promoted the formation of organized and growth-arrested structures with basal polarity, and suppressed oncogenic pathways. Unexpectedly and importantly, we found that unlike reported literature, in 3D the differences between “normal” and malignant phenotypes could not be explained by HIF-1α/2α, AMPK, or mTOR pathways. Loss of epithelial integrity involved activation of RAP1 via exchange protein directly activated by cAMP (EPAC), involving also O-linked N-acetylglucosamine modification downstream of the hexosamine biosynthetic pathway. The former, in turn, was mediated by pyruvate kinase M2 (PKM2) interaction with soluble adenylyl cyclase. Our findings show that increased glucose uptake activates known oncogenic pathways to induce malignant phenotype, and provide possible targets for diagnosis and therapeutics.

Authors

Yasuhito Onodera, Jin-Min Nam, Mina J. Bissell

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Figure 1

Reversion of malignant phenotype in 3D cultures sheds light on the importance of glucose uptake and metabolism in inducing oncogenic signaling.

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Reversion of malignant phenotype in 3D cultures sheds light on the impor...
(AE) S1, T4-2, and reverted T4-2 cells were cultured in 3D lrECM with signaling inhibitors. (A) Experimental scheme. (B) Glucose uptake (black bars) and lactate release (white bars). (C) Western blot of proteins related to these functions. (D) Relative oxygen consumption rate. (E) Western blot of PDC components. Lamin A/C served as a control for both C and E. (FK) S1 and T4-2 cells were cultured in 3D lrECM with or without 4 mM 2DG. (F) Phase-contrast and confocal immunofluorescence (IF; inset) images. Green, α6 integrin; red, nuclei (DAPI). Scale bars: 20 μm. (G) Cell number at the colony midsection (black bars) and EdU incorporation per cell (white bars). (H) Percent colonies with basal polarity. (I) Glucose uptake (black bars) and lactate release (white bars). (J) Relative oxygen consumption rate. (K) Western blot of signaling intermediates, GLUT3, metabolic enzymes, and other proteins related to — or influenced by — glucose metabolism. In B, D, and GJ, data are mean ± SD of triplicate experiments.