Heparan sulfate sulfatase SULF2 regulates PDGFRα signaling and growth in human and mouse malignant glioma
Joanna J. Phillips, … , David H. Rowitch, Zena Werb
Joanna J. Phillips, … , David H. Rowitch, Zena Werb
Published February 1, 2012
Citation Information: J Clin Invest. 2012;122(3):911-922. https://doi.org/10.1172/JCI58215.
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Research Article Neuroscience

Heparan sulfate sulfatase SULF2 regulates PDGFRα signaling and growth in human and mouse malignant glioma

Abstract

Glioblastoma (GBM), a uniformly lethal brain cancer, is characterized by diffuse invasion and abnormal activation of multiple receptor tyrosine kinase (RTK) signaling pathways, presenting a major challenge to effective therapy. The activation of many RTK pathways is regulated by extracellular heparan sulfate proteoglycans (HSPG), suggesting these molecules may be effective targets in the tumor microenvironment. In this study, we demonstrated that the extracellular sulfatase, SULF2, an enzyme that regulates multiple HSPG-dependent RTK signaling pathways, was expressed in primary human GBM tumors and cell lines. Knockdown of SULF2 in human GBM cell lines and generation of gliomas from Sulf2–/– tumorigenic neurospheres resulted in decreased growth in vivo in mice. We found a striking SULF2 dependence in activity of PDGFRα, a major signaling pathway in GBM. Ablation of SULF2 resulted in decreased PDGFRα phosphorylation and decreased downstream MAPK signaling activity. Interestingly, in a survey of SULF2 levels in different subtypes of GBM, the proneural subtype, characterized by aberrations in PDGFRα, demonstrated the strongest SULF2 expression. Therefore, in addition to its potential as an upstream target for therapy of GBM, SULF2 may help identify a subset of GBMs that are more dependent on exogenous growth factor–mediated signaling. Our results suggest the bioavailability of growth factors from the microenvironment is a significant contributor to tumor growth in a major subset of human GBM.

Authors

Joanna J. Phillips, Emmanuelle Huillard, Aaron E. Robinson, Anna Ward, David H. Lum, Mei-Yin Polley, Steven D. Rosen, David H. Rowitch, Zena Werb

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Figure 7

Decreased tumor cell viability conferred by knockdown of SULF2 and inhibition of PDGFR signaling.

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Decreased tumor cell viability conferred by knockdown of SULF2 and inhib...
(A) PDGFRα phosphorylation is decreased by imatinib mesylate (9 μM) in both scrambled shRNA control and SULF2-A shRNA–containing cells by Western blot. (B) Knockdown of SULF2 in combination with inhibition of PDGFRα by imatinib mesylate (9 μM) results in decreased cell viability. This effect was not observed with inhibition of EGFR signaling by AG1478 (10 μM). *P < 0.005. (C) Overexpression of mouse SULF2 (mSULF2) in control and SULF2-A shRNA–containing cells by Western blot. (D) Overexpression of mSULF2 restores PDGFRα activity in cells with knockdown of human SULF2 in an imatinib mesylate–dependent manner. All data are representative of 2 independent experiments done in quadruplicate, and data are presented as mean ± SEM. C, scrambled shRNA control; S2, SULF2-A shRNA.