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    Título
    Targeting metabolic plasticity in glioma stem cells in vitro and in vivo through specific inhibition of c-Src by TAT-Cx43266-283
    Autor(es)
    Gutiérrez Pelaz, SaraUSAL authority ORCID
    Jaraíz-Rodríguez, Myriam
    Álvarez Vázquez, AndreaUSAL authority ORCID
    Talaverón Aguilocho, RocíoUSAL authority ORCID
    García Vicente, LauraUSAL authority ORCID
    Flores-Hernández, Raquel
    Gómez de Cedrón, Marta
    Tabernero, María Dolores
    Ramírez de Molina, Ana
    Lillo Delgado, María ConcepciónUSAL authority ORCID
    Medina Jiménez, José MaríaUSAL authority ORCID
    Tabernero Urbieta, María AránzazuUSAL authority
    Palabras clave
    Cancer metabolism
    Brain tumour
    Connexin
    Glioblastoma stem cells
    GLUT-3
    Hexokinase-2
    Clasificación UNESCO
    3207.13 Oncología
    2407 Biología Celular
    2490 Neurociencias
    Fecha de publicación
    2020-11-02
    Resumen
    Background: Glioblastoma is the most aggressive primary brain tumour and has a very poor prognosis. Inhibition of c-Src activity in glioblastoma stem cells (GSCs, responsible for glioblastoma lethality) and primary glioblastoma cells by the peptide TAT-Cx43266-283 reduces tumorigenicity, and boosts survival in preclinical models. Because c-Src can modulate cell metabolism and several reports revealed poor clinical efficacy of various antitumoral drugs due to metabolic rewiring in cancer cells, here we explored the inhibition of advantageous GSC metabolic plasticity by the c-Src inhibitor TAT-Cx43266-283. Methods: Metabolic impairment induced by the c-Src inhibitor TAT-Cx43266-283 in vitro was assessed by fluorometry, western blotting, immunofluorescence, qPCR, enzyme activity assays, electron microscopy, Seahorse analysis, time-lapse imaging, siRNA, and MTT assays. Protein expression in tumours from a xenograft orthotopic glioblastoma mouse model was evaluated by immunofluorescence. Findings: TAT-Cx43266-283 decreased glucose uptake in human GSCs and reduced oxidative phosphorylation without a compensatory increase in glycolysis, with no effect on brain cell metabolism, including rat neurons, human and rat astrocytes, and human neural stem cells. TAT-Cx43266-283 impaired metabolic plasticity, reducing GSC growth and survival under different nutrient environments. Finally, GSCs intracranially implanted with TAT-Cx43266-283 showed decreased levels of important metabolic targets for cancer therapy, such as hexokinase-2 and GLUT-3. Interpretation: The reduced ability of TAT-Cx43266-283-treated GSCs to survive in metabolically challenging settings, such as those with restricted nutrient availability or the ever-changing in vivo environment, allows us to conclude that the advantageous metabolic plasticity of GSCs can be therapeutically exploited through the specific and cell-selective inhibition of c-Src by TAT-Cx43266-283.
    URI
    https://hdl.handle.net/10366/154967
    ISSN
    2352-3964
    DOI
    10.1016/j.ebiom.2020.103134
    Versión del editor
    https://doi.org/10.1016/j.ebiom.2020.103134
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    • INCyL. Unidad de Excelencia iBRAINS-IN-CyL [141]
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