[No authors listed]
Glioblastoma harbors frequent alterations in receptor tyrosine kinases, phosphatidylinositolâ3 kinase (PI3K) and phosphatase and tensin homolog (PTEN) that dysregulate phospholipid signaling driven tumor proliferation and therapeutic resistance. Myristoylated alanineârich Câkinase substrate (MARCKS) is a 32 kDa intrinsically unstructured protein containing a polybasic (+13) effector domain (ED), which regulates its electrostatic sequestration of phospholipid phosphatidylinositol (4,5)âbisphosphate (PIP2), and its binding to phosphatidylserine, calcium/calmodulin, filamentous actin, while also serving as a nuclear localization sequence. MARCKS ED is phosphorylated by protein and Rhoâassociated protein kinase (ROCK) kinases; however, the impact of MARCKS on glioblastoma growth and radiation sensitivity remains undetermined. In the present study, using a tetracyclineâinducible system in PTENânull U87 cells, we demonstrate that MARCKS overexpression suppresses growth and enhances radiation sensitivity in vivo. A new image cytometer, Xcyto10, was utilized to quantify differences in MARCKS ED phosphorylation on localization and its association with filamentous actin. The overexpression of the nonâphosphorylatable ED mutant exerted growthâsuppressive and radiationâsensitizing effects, while the pseudoâphosphorylated ED mutant exhibited an enhanced colony formation and clonogenic survival ability. The identification of MARCKS proteinâprotein interactions using coâimmunoprecipitation coupled with tandem mass spectrometry revealed novel MARCKSâassociated proteins, including importinâβ and ku70. On the whole, the findings of this study suggest that the determination of the MARCKS ED phosphorylation status is essential to understanding the impact of MARCKS on cancer progression.
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