Intensified mitophagy in skeletal muscle with aging is downregulated by PGC-1alpha overexpression in vivo.

6533b86cfe1ef96bd12c8058

RESEARCH PRODUCT

Intensified mitophagy in skeletal muscle with aging is downregulated by PGC-1alpha overexpression in vivo.

Li Li Ji Chounghun Kang Jose Viña Mari Carmen Gomez-cabrera Dongwook Yeo

subject

0301 basic medicine Aging Ubiquitin-Protein Ligases PINK1 Mitochondrion Biochemistry Mitochondrial Dynamics GTP Phosphohydrolases 03 medical and health sciences Mice 0302 clinical medicine In vivo Physiology (medical)Mitophagy medicine Animals Muscle Skeletal Chemistry Mitophagy Skeletal muscle Transfection medicine.disease Peroxisome Proliferator-Activated Receptor Gamma Coactivator 1-alpha Muscle atrophy Cell biology Mitochondria Oxidative Stress 030104 developmental biology medicine.anatomical_structure Gene Expression Regulation Sarcopenia Beclin-1 medicine.symptom Protein Kinases 030217 neurology & neurosurgery

description

Mitochondrial dysfunction plays an important role in the etiology of age-related muscle atrophy known as sarcopenia. PGC-1α is positioned at the center of crosstalk in regulating mitochondrial quality control, but its role in mitophagy in aged skeletal muscle is currently unclear. The present study investigated the effects of aging and PGC-1α overexpression via in vivo DNA transfection on key mitophagy protein markers, as well as mitochondrial dynamics related proteins, metabolic function and antioxidant capacity in mouse muscle. C57BL/6J mice at the age of 2 mo (young, Y; N = 14) and 24 mo (old, O; N = 14) were transfected in vivo with either PGC-1α DNA (OE, N = 7) or GFP (N = 7) into the tibialis anterior (TA) muscle followed by electroporation. PINK1 and Parkin protein contents were 3.6 and 1.4-fold higher (P  0.01), whereas mitochondrial ubiquitination (Ub) increased 1.5-fold (P  0.05), in O vs. Y mice. PGC-1 OE suppressed PINK and Parkin protein levels by 50-60% (P  0.01), and decreased Ub by 20% (P  0.05) in old mice. Aging significantly increased the protein content of LC3II (30%, P  0.05), p62 (42%, P  0.05), RheB (5.5-fold, P  0.01), Beclin-1 (3-fold, P  0.01) and Mfn2 (~4-fold, P  0.01) in the TA muscle. However, these age-related increases in mitophagy markers were attenuated by PGC-1α OE. Furthermore, aging dramatically increased Fis-1 protein content by 14-fold (P  0.01), along with a severe reduction of citrate synthase activity (64%, P  0.01) and cytochrome c oxidase subunit IV (COXIV) protein content (85%, P  0.01). PGC-1α OE mitigated the age effects on Fis-1 and Drp-1 (P  0.05). Moreover, PGC-1α OE enhanced mitochondrial oxidative function and antioxidant enzyme activities, and decreased lipid peroxidation and inner membrane damage found in old mice (P  0.01). In summary, our data demonstrate that mitophagy protein expression in skeletal muscle was enhanced at old age driven possibly by increased mitochondrial dysfunction, damage, and fission. PGC-1α OE was effective in ameliorating mitochondrial deficits but did not restore muscle fiber atrophy.

year	journal	country	edition	language
2018-08-02	Free radical biologymedicine

10.1016/j.freeradbiomed.2018.10.456 https://pubmed.ncbi.nlm.nih.gov/30395971