CIP2A induces PKM2 tetramer formation and oxidative phosphorylation in non-small cell lung cancer

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Li-Jun Liang
Fu-Ying Yang
Di Wang
Yan-Fei Zhang
Hong Yu
Zheng Wang
Bei-Bei Sun
Yu-Tao Liu
Gui-Zhen Wang
Guang-Biao Zhou
机构
[1] Chinese Academy of Medical Sciences and Peking Union Medical College,State Key Laboratory of Molecular Oncology & Department of Medical Oncology, National Cancer Center/National Clinical Research Center for Cancer/Cancer Hospital
[2] Zhejiang University,Department of Thoracic Surgery, Second Affiliated Hospital, School of Medicine
[3] Peking Union Medical College Hospital,Department of Clinical Laboratory
[4] Chinese Academy of Medical Sciences and Peking Union Medical College,Department of Basic Medicine
[5] Anhui Medical College,Department of Pharmacology
[6] University of Texas Health Science at San Antonio,undefined
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Tumor cells are usually considered defective in mitochondrial respiration, but human non-small cell lung cancer (NSCLC) tumor tissues are shown to have enhanced glucose oxidation relative to adjacent benign lung. Here, we reported that oncoprotein cancerous inhibitor of protein phosphatase 2A (CIP2A) inhibited glycolysis and promoted oxidative metabolism in NSCLC cells. CIP2A bound to pyruvate kinase M2 (PKM2) and induced the formation of PKM2 tetramer, with serine 287 as a novel phosphorylation site essential for PKM2 dimer-tetramer switching. CIP2A redirected PKM2 to mitochondrion, leading to upregulation of Bcl2 via phosphorylating Bcl2 at threonine 69. Clinically, CIP2A level in tumor tissues was positively correlated with the level of phosphorylated PKM2 S287. CIP2A-targeting compounds synergized with glycolysis inhibitor in suppressing cell proliferation in vitro and in vivo. These results indicated that CIP2A facilitates oxidative phosphorylation by promoting tetrameric PKM2 formation, and targeting CIP2A and glycolysis exhibits therapeutic potentials in NSCLC.
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