Unbalancing cAMP and Ras/MAPK pathways as a therapeutic strategy for cutaneous neurofibromas
Helena Mazuelas, Miriam Magallón-Lorenz, Itziar Uriarte-Arrazola, Alejandro Negro, Inma Rosas, Ignacio Blanco, Elisabeth Castellanos, Conxi Lázaro, Bernat Gel, Meritxell Carrió, Eduard Serra
Helena Mazuelas, Miriam Magallón-Lorenz, Itziar Uriarte-Arrazola, Alejandro Negro, Inma Rosas, Ignacio Blanco, Elisabeth Castellanos, Conxi Lázaro, Bernat Gel, Meritxell Carrió, Eduard Serra
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Research Article Cell biology Genetics

Unbalancing cAMP and Ras/MAPK pathways as a therapeutic strategy for cutaneous neurofibromas

Abstract

Cutaneous neurofibromas (cNFs) are benign Schwann cell (SC) tumors arising from subepidermal glia. Individuals with neurofibromatosis type 1 (NF1) may develop thousands of cNFs, which greatly affect their quality of life. cNF growth is driven by the proliferation of NF1–/– SCs and their interaction with the NF1+/– microenvironment. We analyzed the crosstalk between human cNF-derived SCs and fibroblasts (FBs), identifying an expression signature specific to the SC-FB interaction. We validated the secretion of proteins involved in immune cell migration, suggesting a role of SC-FB crosstalk in immune cell recruitment. The signature also captured components of developmental signaling pathways, including the cAMP elevator G protein–coupled receptor 68 (GPR68). Activation of Gpr68 by ogerin in combination with the MEK inhibitor (MEKi) selumetinib reduced viability and induced differentiation and death of human cNF-derived primary SCs, a result corroborated using an induced pluripotent stem cell–derived 3D neurofibromasphere model. Similar results were obtained using other Gpr68 activators or cAMP analogs/adenylyl cyclase activators in combination with selumetinib. Interestingly, whereas primary SC cultures restarted their proliferation after treatment with selumetinib alone was stopped, the combination of ogerin-selumetinib elicited a permanent halt on SC expansion that persisted after drug removal. These results indicate that unbalancing the Ras and cAMP pathways by combining MEKi and cAMP elevators could be used as a potential treatment for cNFs.

Authors

Helena Mazuelas, Miriam Magallón-Lorenz, Itziar Uriarte-Arrazola, Alejandro Negro, Inma Rosas, Ignacio Blanco, Elisabeth Castellanos, Conxi Lázaro, Bernat Gel, Meritxell Carrió, Eduard Serra

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Figure 6

Selumetinib-ogerin cotreatment leads to differentiation and increased cell death in cNF-derived primary SCs.

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Selumetinib-ogerin cotreatment leads to differentiation and increased ce...
(A) Effect of selumetinib and ogerin treatments and cotreatments on cell viability in cNF-derived primary SC cultures. Cell viability was monitored over 72 hours using the RealTime-Glo MT Cell Viability Assay. Three different SC cultures were used. Mean is represented, and data are expressed as relative viability to DMSO-treated control cells. (B) Effect of selumetinib treatments and selumetinib-ogerin cotreatments on cell death in cNF-derived primary SC cultures. Cell death was monitored using the flow cytometry Annexin V Apoptosis Detection Kit. Data are expressed as the percentage of cells in early and late apoptosis per condition in 3 different SC cultures. Median is represented. One-tailed unpaired t test (P ≤ 0.05). (C) Immunocytochemical analysis for S100B and MPZ in SC-treated cultures. DAPI was used to stain cell nuclei. Scale bars: 200 μm (S100B), except in higher-magnification views; 100 μm (MPZ). (D) Effect of selumetinib and ogerin or the ogerin-analog PAM71 treatment and cotreatment on cell viability in cNF-derived primary SC cultures. Three SC cultures were used. Mean is represented, and data are expressed as relative viability to DMSO-treated control cells. (E) Effect of selumetinib and the cAMP analog 8CPT (top) or forskolin (F; bottom) on cell viability in cNF-derived primary SC cultures. Three different SC cultures were used. Mean is represented, and data are expressed as relative viability to DMSO-treated control cells. (F) Immunocytochemical analysis for MPZ in treated SC cultures. DAPI was used to stain cell nuclei. Scale bars: 100 μm.