1. Academic Validation
  2. AKT1 Promotes Tumorigenesis and Metastasis by Directly Phosphorylating Hexokinases

AKT1 Promotes Tumorigenesis and Metastasis by Directly Phosphorylating Hexokinases

  • J Cell Biochem. 2024 Jun 11. doi: 10.1002/jcb.30613.
Yuan Yu 1 Shuqing Wang 2 Yaqi Wang 3 Qianyi Zhang 1 Lina Zhao 1 Yang Wang 1 Jinghua Wu 4 Liyuan Han 4 Junli Wang 1 Jimin Guo 1 Jiarui Xue 1 Fenglin Dong 1 Jing Hua Zhang 5 Liu Zhang 1 Yan Liu 1 6 Guogang Shi 7 Xiaojun Zhang 7 Yufeng Li 6 8 Jingwu Li 6 8 9
Affiliations

Affiliations

  • 1 College of Life Science, North China University of Science and Technology, Tangshan, China.
  • 2 Hospital of North China University of Science and Technology, Tangshan, China.
  • 3 Department of the First Breast Surgery, Tangshan People's Hospital, Tangshan, China.
  • 4 Department of Inspection, North China University of Science and Technology Affiliated Tangshan Maternal and Child Health Hospital, Tangshan, China.
  • 5 Department of Clinical Laboratory, North China University of Science and Technology Affiliated Tangshan Maternal and Child Health Hospital, Tangshan, China.
  • 6 Hebei Key Laboratory of Molecular Oncology, Tangshan, Hebei, China.
  • 7 Department of Oncology, People's Hospital of Zunhua, Tangshan, China.
  • 8 The Cancer Institute, Tangshan People's Hospital, Tangshan, Hebei, China.
  • 9 Tangshan Key Laboratory of Cancer Prevention and Treatment, Tangshan, Hebei, China.
Abstract

The importance of protein kinase B (Akt) in tumorigenesis and development is well established, but its potential regulation of metabolic reprogramming via phosphorylation of the Hexokinase (HK) isozymes remains unclear. There are two HK family members (HK1/2) and three Akt family members (Akt1/2/3), with varied distribution of AKTs exhibiting distinct functions in different tissues and cell types. Although Akt is known to phosphorylate HK2 at threonine 473, AKT-mediated phosphorylation of HK1 has not been reported. We examined direct binding and phosphorylation of HK1/2 by Akt1 and identified the phosphorylation modification sites using coimmunoprecipitation, glutathione pull-down, western blotting, and in vitro kinase assays. Regulation of HK activity through phosphorylation by Akt1 was also examined. Uptake of 2-[1,2-3H]-deoxyglucose and production of lactate were investigated to determine whether Akt1 regulates glucose metabolism by phosphorylating HK1/2. Functional assays, immunohistochemistry, and tumor experiments in mice were performed to investigate whether AKT1-mediated regulation of tumor development is dependent on its kinase activity and/or the involvement of HK1/2. Akt interacted with and phosphorylated HK1 and HK2. Serine phosphorylation significantly increased Akt kinase activity, thereby enhancing glycolysis. Mechanistically, the phosphorylation of HK1 at serine 178 (S178) by Akt significantly decreased the Km and enhanced the Vmax by interfering with the formation of HK1 dimers. Mutations in the Akt phosphorylation sites of HK1 or HK2 significantly abrogated the stimulatory characteristics of Akt on glycolysis, tumorigenesis, and cell migration, invasion, proliferation, and metastasis. HK1-S178 phosphorylation levels were significantly correlated with the occurrence and metastasis of different types of clinical tumors. We conclude that Akt not only regulates tumor glucose metabolism by directly phosphorylating HK1 and HK2, but also plays important roles in tumor progression, proliferation, and migration.

Keywords

AKT1; HK1; HK2.

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