Deletion of PRKAA triggers mitochondrial fission by inhibiting the autophagy-dependent degradation of DNM1L

Qilong Wang; Shengnan Wu; Huaiping Zhu; Ye Ding; Xiaoyan Dai; Changhan Ouyang; Young-Min Han; Zhonglin Xie; Ming-Hui Zou

doi:10.1080/15548627.2016.1263776

Deletion of PRKAA triggers mitochondrial fission by inhibiting the autophagy-dependent degradation of DNM1L

Autophagy. 2017 Feb;13(2):404-422. doi: 10.1080/15548627.2016.1263776. Epub 2017 Jan 13.

Authors

Qilong Wang¹, Shengnan Wu¹, Huaiping Zhu¹, Ye Ding¹, Xiaoyan Dai¹, Changhan Ouyang¹, Young-Min Han¹, Zhonglin Xie¹, Ming-Hui Zou¹

Affiliation

¹ a Center for Molecular and Translational Medicine, Georgia State University , Atlanta , GA USA.

Abstract

PRKAA (protein kinase, AMP-activated, α catalytic subunit) regulates mitochondrial biogenesis, function, and turnover. However, the molecular mechanisms by which PRKAA regulates mitochondrial dynamics remain poorly characterized. Here, we report that PRKAA regulated mitochondrial fission via the autophagy-dependent degradation of DNM1L (dynamin 1-like). Deletion of Prkaa1/AMPKα1 or Prkaa2/AMPKα2 resulted in defective autophagy, DNM1L accumulation, and aberrant mitochondrial fragmentation in the mouse aortic endothelium. Furthermore, autophagy inhibition by chloroquine treatment or ATG7 small interfering RNA (siRNA) transfection, upregulated DNM1L expression and triggered DNM1L-mediated mitochondrial fragmentation. In contrast, autophagy activation by overexpression of ATG7 or chronic administration of rapamycin, the MTOR inhibitor, promoted DNM1L degradation and attenuated mitochondrial fragmentation in Prkaa2-deficient (prkaa2^-/-) mice, suggesting that defective autophagy contributes to enhanced DNM1L expression and mitochondrial fragmentation. Additionally, the autophagic receptor protein SQSTM1/p62, which bound to DNM1L and led to its translocation into the autophagosome, was involved in DNM1L degradation by the autophagy-lysosome pathway. Gene silencing of SQSTM1 markedly reduced the association between SQSTM1 and DNM1L, impaired the degradation of DNM1L, and enhanced mitochondrial fragmentation in PRKAA-deficient endothelial cells. Finally, the genetic (DNM1L siRNA) or pharmacological (mdivi-1) inhibition of DNMA1L ablated mitochondrial fragmentation in the mouse aortic endothelium and prevented the acetylcholine-induced relaxation of isolated mouse aortas. This suggests that aberrant DNM1L is responsible for enhanced mitochondrial fragmentation and endothelial dysfunction in prkaa knockout mice. Overall, our results show that PRKAA deletion promoted mitochondrial fragmentation in vascular endothelial cells by inhibiting the autophagy-dependent degradation of DNM1L.

Keywords: AMPK; DNM1L; PRKAA/AMPK catalytic subunit α; autophagy; endothelial dysfunction; mitochondrial fission.

MeSH terms

AMP-Activated Protein Kinases / metabolism*
Animals
Aorta / metabolism
Aorta / ultrastructure
Autophagy* / drug effects
Cell Separation
Dynamins / metabolism*
Endothelium, Vascular / drug effects
Endothelium, Vascular / metabolism
GTP Phosphohydrolases / metabolism*
Gene Deletion*
Human Umbilical Vein Endothelial Cells / drug effects
Human Umbilical Vein Endothelial Cells / metabolism
Humans
Mice, Inbred C57BL
Microtubule-Associated Proteins / metabolism*
Mitochondrial Dynamics* / drug effects
Mitochondrial Proteins / metabolism*
Phosphorylation / drug effects
Phosphoserine / metabolism
Proteolysis* / drug effects
Sequestosome-1 Protein / metabolism
Sirolimus / administration & dosage
Sirolimus / pharmacology
Vasodilation / drug effects

Substances

Microtubule-Associated Proteins
Mitochondrial Proteins
SQSTM1 protein, human
Sequestosome-1 Protein
Phosphoserine
PRKAA2 protein, human
AMP-Activated Protein Kinases
PRKAA1 protein, human
GTP Phosphohydrolases
DNM1L protein, human
Dnm1l protein, mouse
Dynamins
Sirolimus