Proteolytic activation of angiomotin by DDI2 promotes angiogenesis.
Yu WangYuwen ZhuYebin WangYue ChangFang GengMingyue MaYuan GuAijuan YuRui ZhuPengcheng YuZhao ShaSixian QiJian LiWencao ZhaoWeijun PanRuilin ZhangFa-Xing YuPublished in: The EMBO journal (2023)
The scaffolding protein angiomotin (AMOT) is indispensable for vertebrate embryonic angiogenesis. Here, we report that AMOT undergoes cleavage in the presence of lysophosphatidic acid (LPA), a lipid growth factor also involved in angiogenesis. AMOT cleavage is mediated by aspartic protease DNA damage-inducible 1 homolog 2 (DDI2), and the process is tightly regulated by a signaling axis including neurofibromin 2 (NF2), tankyrase 1/2 (TNKS1/2), and RING finger protein 146 (RNF146), which induce AMOT membrane localization, poly ADP ribosylation, and ubiquitination, respectively. In both zebrafish and mice, the genetic inactivation of AMOT cleavage regulators leads to defective angiogenesis, and the phenotype is rescued by the overexpression of AMOT-CT, a C-terminal AMOT cleavage product. In either physiological or pathological angiogenesis, AMOT-CT is required for vascular expansion, whereas uncleavable AMOT represses this process. Thus, our work uncovers a signaling pathway that regulates angiogenesis by modulating a cleavage-dependent activation of AMOT.
Keyphrases
- endothelial cells
- signaling pathway
- vascular endothelial growth factor
- growth factor
- dna damage
- dna binding
- wound healing
- computed tomography
- oxidative stress
- transcription factor
- type diabetes
- immune response
- adipose tissue
- magnetic resonance imaging
- dual energy
- epithelial mesenchymal transition
- image quality
- magnetic resonance
- gene expression
- contrast enhanced
- skeletal muscle
- dna methylation
- positron emission tomography
- copy number
- amino acid
- inflammatory response
- insulin resistance
- toll like receptor