Affiliation:
1. Departments of Inflammation and Immunity, Gastroenterology & Hepatology Cleveland Clinic Cleveland OH USA
2. KEM Hospital Seth GS Medical College Mumbai India
3. Respiratory Medicine Cleveland Clinic Cleveland Ohio USA
4. Quantitative Health Cleveland Clinic Cleveland Ohio USA
5. Department of Radiation Oncology Philadelphia PA USA
6. Proteomics and Metabolomics Core, Lerner Research Institute Cleveland Clinic Cleveland OH USA
7. Department of Molecular and Integrative Physiology University of Michigan Ann Arbor MI USA
Abstract
AbstractHypoxia‐inducible factor (HIF)‐1α is continuously synthesized and degraded in normoxia. During hypoxia, HIF1α stabilization restricts cellular/mitochondrial oxygen utilization. Cellular stressors can stabilize HIF1α even during normoxia. However, less is known about HIF1α function(s) and sex‐specific effects during normoxia in the basal state. Since skeletal muscle is the largest protein store in mammals and protein homeostasis has high energy demands, we determined HIF1α function at baseline during normoxia in skeletal muscle. Untargeted multiomics data analyses were followed by experimental validation in differentiated murine myotubes with loss/gain of function and skeletal muscle from mice without/with post‐natal muscle‐specific Hif1a deletion (Hif1amsd). Mitochondrial oxygen consumption studies using substrate, uncoupler, inhibitor, titration protocols; targeted metabolite quantification by gas chromatography–mass spectrometry; and post‐mitotic senescence markers using biochemical assays were performed. Multiomics analyses showed enrichment in mitochondrial and cell cycle regulatory pathways in Hif1a deleted cells/tissue. Experimentally, mitochondrial oxidative functions and ATP content were higher with less mitochondrial free radical generation with Hif1a deletion. Deletion of Hif1a also resulted in higher concentrations of TCA cycle intermediates and HIF2α proteins in myotubes. Overall responses to Hif1amsd were similar in male and female mice, but changes in complex II function, maximum respiration, Sirt3 and HIF1β protein expression and muscle fibre diameter were sex‐dependent. Adaptive responses to hypoxia are mediated by stabilization of constantly synthesized HIF1α. Despite rapid degradation, the presence of HIF1α during normoxia contributes to lower mitochondrial oxidative efficiency and greater post‐mitotic senescence in skeletal muscle. In vivo responses to HIF1α in skeletal muscle were differentially impacted by sex.
imageKey points
Hypoxia‐inducible factor ‐1α (HIF1α), a critical transcription factor, undergoes continuous synthesis and proteolysis, enabling rapid adaptive responses to hypoxia by reducing mitochondrial oxygen consumption.
In mammals, skeletal muscle is the largest protein store which is determined by a balance between protein synthesis and breakdown and is sensitive to mitochondrial oxidative function.
To investigate the functional consequences of transient HIF1α expression during normoxia in the basal state, myotubes and skeletal muscle from male and female mice with HIF1α knockout were studied using complementary multiomics, biochemical and metabolite assays.
HIF1α knockout altered the electron transport chain, mitochondrial oxidative function, signalling molecules for protein homeostasis, and post‐mitotic senescence markers, some of which were differentially impacted by sex.
The cost of rapid adaptive responses mediated by HIF1α is lower mitochondrial oxidative efficiency and post‐mitotic senescence during normoxia.