Parkin is a critical player in the effects of caffeine over mitochondrial quality control pathways during skeletal muscle regeneration in mice

Author:

Esteca M. V.1,Divino I. A.1,Vieira da Silva A. L.1,Severino M. B.12,Braga R. R.3,Ropelle E. R.3,Simabuco F. M.24,Baptista I. L.1ORCID

Affiliation:

1. Laboratory of Cell and Tissue Biology, School of Applied Sciences University of Campinas Limeira Brazil

2. Multidisciplinarity Laboratory of Food and Health, School of Applied Sciences University of Campinas Limeira Brazil

3. Laboratory of Molecular Biology of Exercise, School of Applied Sciences University of Campinas Limeira Brazil

4. Department of Biochemistry Federal University of São Paulo São Paulo Brazil

Abstract

AbstractAimThis study aimed to investigate the effects of caffeine on pathways associated with mitochondrial quality control and mitochondrial capacity during skeletal muscle regeneration, focusing on the role of Parkin, a key protein involved in mitophagy.MethodsWe used in vitro C2C12 myoblast during differentiation with and without caffeine in the medium, and we evaluated several markers of mitochondrial quality control pathways and myotube growth. In vivo experiments, we used C57BL/6J (WT) and Parkintm1Shn lineage (Parkin−/−) mice and injured tibial anterior muscle. The mice regenerated TA muscle for 3, 10, and 21 days with or without caffeine ingestion. TA muscle was used to analyze the protein content of several markers of mitochondrial quality pathways, muscle satellite cell differentiation, and protein synthesis. Furthermore, it analyzed mtDNA, mitochondrial respiration, and myofiber growth.ResultsC2C12 differentiation experiments showed that caffeine decreased Parkin content, potentially leading to increased DRP1 and PGC‐1α content and altered mitochondrial population, thereby enhancing growth capacity. Using Parkin−/− mice, we found that caffeine intake during the regenerative process induces an increase in AMPKα phosphorylation and PGC‐1α and TFAM content, changes that were partly Parkin‐dependent. In addition, the absence of Parkin potentiates the ergogenic effect of caffeine by increasing mitochondrial capacity and myotube growth. Those effects are related to increased ATF4 content and activation of protein synthesis pathways, such as increased 4E‐BP1 phosphorylation.ConclusionThese findings demonstrate that caffeine ingestion changes mitochondrial quality control during skeletal muscle regeneration, and Parkin is a central player in those mechanisms.

Funder

Conselho Nacional de Desenvolvimento Científico e Tecnológico

Fundação de Amparo à Pesquisa do Estado de São Paulo

Publisher

Wiley

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