4.7 Article

Ablation of Proton/Glucose Exporter SLC45A2 Enhances Melanosomal Glycolysis to Inhibit Melanin Biosynthesis and Promote Melanoma Metastasis

JOURNAL OF INVESTIGATIVE DERMATOLOGY (2022)

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Journal

JOURNAL OF INVESTIGATIVE DERMATOLOGY
Volume 142, Issue 10, Pages 2744-+

Publisher

ELSEVIER SCIENCE INC
DOI: 10.1016/j.jid.2022.04.008

Keywords

phosphatidylinositol 3-kinase; PMC; primary melanocyte; Tyr; tyrosinase

Categories

Dermatology

Funding

  1. National Natural Science Foundation of China [32130048, 92157301, 31971085, 91857108]
  2. Ministry of Science and Technology of China National Key RD Programs [2018YFA0506903]
  3. Nation Science and Technology Major Projects for Major New Drugs Innovation and Development [2018ZX09711003-004-002]
  4. Tsinghua University Spring Breeze Fund [2021Z99CFY012]
  5. Tsinghua-Foshan Innovation Special Fund [2020THFS0133]

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Sequence variation in SLC45A2 is associated with oculocutaneous albinism type 4 and melanoma susceptibility. The study reveals that SLC45A2 plays a critical role in melanogenesis and melanoma metastasis. Slc45a2-deficient melanocytes have impaired activity of the key melanogenic enzyme tyrosinase due to the acidified cellular environment. SLC45A2 is identified as a proton/glucose exporter in melanosomes, and its deficiency leads to increased acidification of melanosomal pH through enhanced glycolysis. Additionally, Slc45a2 deficiency upregulates glycolytic enzymes and PI3K/AKT signaling, promoting glycolysis-dependent survival and metastasis of melanoma cells.
Sequence variation in SLC45A2 are responsible for oculocutaneous albinism type 4 in many species and are associated with melanoma susceptibility, but the molecular mechanism is unclear. In this study, we used Slc45a2-deficient melanocyte and mouse models to elucidate the roles of SLC45A2 in melanogenesis and melanoma metastasis. We found that the acidified cellular environment impairs the activity of key melanogenic enzyme tyrosinase in Slc45a2-deficient melanocytes. SLC45A2 is identified as a proton/glucose exporter in melanosomes, and its ablation increases the acidification of melanosomal pH through enhanced glycolysis. Intriguingly, 13C-glucose-labeled metabolic flux and biochemical assays show that melanosomes are active glucose-metabolizing organelles, indicating that elevated glycolysis mainly occurs in melanosomes owing to Slc45a2 deficiency. Moreover, Slc45a2 deficiency significantly upregulates the activities of glycolytic enzymes and phosphatidylinositol 3-kinase/protein kinase B signaling to promote glycolysis-dependent survival and metastasis of melanoma cells. Collectively, our study reveals that the proton/glucose exporter SLC45A2 me-diates melanin synthesis and melanoma metastasis primarily by modulating melanosomal glucose metabolism.

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