4.5 Article

KDM5A silencing transcriptionally suppresses the FXYD3-PI3K/AKT axis to inhibit angiogenesis in hepatocellular cancer via miR-433 up-regulation

JOURNAL OF CELLULAR AND MOLECULAR MEDICINE (2021)

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Journal

JOURNAL OF CELLULAR AND MOLECULAR MEDICINE
Volume 25, Issue 8, Pages 4040-4052

Publisher

WILEY
DOI: 10.1111/jcmm.16371

Keywords

angiogenesis; FXYD domain‐ containing ion transport regulator 3; FXYD3; invasion; microRNA‐ 433; migration; miR‐ 433; PI3K; AKT; proliferation

Categories

Cell Biology Medicine, Research & Experimental

Funding

  1. National Natural Science Foundation of China [81972214, 81772932, 81201535, 81302065]
  2. Nantong Science and Technology Project [JC2018125, JC2018010, yyz15026]
  3. Construction of Clinical Medical Center for Tumor Biological Samples in Nantong [HS2016004]
  4. Peak of Six Personnel Foundation in Jiangsu Province [WSW-009]
  5. Jiangsu Provincial University Natural Science Funding [19KJB180021]
  6. Jiangsu 333 Program [BRA2017205]
  7. Nantong Medical Key Talents Training Plan [43]
  8. Wu Jieping Medical Foundation [320.6750.14326]

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This study investigates the role of KDM5A in angiogenesis and mechanisms in HCC, revealing that KDM5A suppresses miR-433 and activates the FXYD3-PI3K-AKT axis to promote HCC progression.
Hepatocellular cancer (HCC) has been reported to belong to one of the highly vascularized solid tumours accompanied with angiogenesis of human umbilical vein endothelial cells (HUVECs). KDM5A, an attractive drug target, plays a critical role in diverse physiological processes. Thus, this study aims to investigate its role in angiogenesis and underlying mechanisms in HCC. ChIP-qPCR was utilized to validate enrichment of H3K4me3 and KDM5A on the promotor region of miR-433, while dual luciferase assay was carried out to confirm the targeting relationship between miR-433 and FXYD3. Scratch assay, transwell assay, Edu assay, pseudo-tube formation assay and mice with xenografted tumours were conducted to investigate the physiological function of KDM5A-miR-433-FXYD3-PI3K-AKT axis in the progression of HCC after loss- and gain-function assays. KDM5A p-p85 and p-AKT were highly expressed but miR-433 was down-regulated in HCC tissues and cell lines. Depletion of KDM5A led to reduced migrative, invasive and proliferative capacities in HCC cells, including growth and a lowered HUVEC angiogenic capacity in vitro. Furthermore, KDM5A suppressed the expression of miR-433 by demethylating H3K4me3 on its promoterregion. miR-433 negatively targeted FXYD3. Depleting miR-433 or re-expressing FXYD3 restores the reduced migrative, invasive and proliferative capacities, and lowers the HUVEC angiogenic capacity caused by silencing KDM5A. Therefore, KDM5A silencing significantly suppresses HCC tumorigenesis in vivo, accompanied with down-regulated miR-433 and up-regulated FXYD3-PI3K-AKT axis in tumour tissues. Lastly, KDM5A activates the FXYD3-PI3K-AKT axis to enhance angiogenesis in HCC by suppressing miR-433.

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