Autophagy signaling in skeletal muscle of infarcted rats

Background: Heart failure (HF)-induced skeletal muscle atrophy is often associated to exercise intolerance and poor prognosis. Better understanding of the molecular mechanisms underlying HF-induced muscle atrophy may contribute to the development of pharmacological strategies to prevent or treat such condition. It has been shown that autophagylysosome system is an important mechanism for maintenance of muscle mass. However, its role in HF-induced myopathy has not been addressed yet. Therefore, the aim of the present study was to evaluate autophagy signaling in myocardial infarction (MI)-induced muscle atrophy in rats.\ud Methods/Principal Findings: Wistar rats underwent MI or Sham surgeries, and after 12 weeks were submitted toechocardiography, exercise tolerance and histology evaluations. Cathepsin L activity and expression of autophagy-related\ud genes and proteins were assessed in soleus and plantaris muscles by fluorimetric assay, qRT-PCR and immunoblotting, respectively. MI rats displayed exercise intolerance, left ventricular dysfunction and dilation, thereby suggesting the presence of HF. The key findings of the present study were: a) upregulation of autophagy-related genes (GABARAPL1, ATG7, BNIP3, CTSL1 and LAMP2) was observed only in plantaris while muscle atrophy was observed in both soleus and plantaris muscles, and b) Cathepsin L activity, Bnip3 and Fis1 protein levels, and levels of lipid hydroperoxides were increased\ud specifically in plantaris muscle of MI rats.\ud Conclusions: Altogether our results provide evidence for autophagy signaling regulation in HF-induced plantaris atrophy but not soleus atrophy. Therefore, autophagy-lysosome system is differentially regulated in atrophic muscles comprising different fiber-types and metabolic characteristics.Fundação de Amparo à Pesquisa do Estado de São Paulo, Brazil (FAPESP #2010/14567-4).FAPESP (#2010/50048-1)Conselho Nacional de Pesquisa e Desenvolvimento (CNPq #302201/2011-4

Aerobic exercise-induced mitochondrial adaptation: unraveling novel molecular mechanisms

O aumento da capacidade oxidativa é considerado o fator central dos seus benefícios à saúde induzidos pelo exercício físico aeróbio (EFA). A musculatura esquelética é um dos tecidos mais envolvidos na realização de exercícios físicos, com capacidade notável de adaptação metabólica e estrutural frente ao estímulo mecânico. Os músculos esqueléticos são ricos em mitocôndrias e altamente dependentes da fosforilação oxidativa para a produção energia. Assim, o aumento da capacidade aeróbia induzido pelo EFA ocorre grande parte em função de adaptações mitocondriais. Inúmeros estudos demonstram a capacidade do EFA em induzir biogênese mitocondrial, onde o coativador de transcrição PGC-1?1 atua coordenando a expressão de genes nucleares e mitocondriais no contexto do EFA. No entanto, animais com deleção de PGC- 1?1 no músculo esquelético ainda apresentam remodelamento mitocondrial importante após período de treinamento físico aeróbio, evidenciando a existência de mecanismos ainda desconhecidos. Embora a formação de novas mitocôndrias seja fundamental, a manutenção de mitocôndrias saudáveis por meio de mecanismos de controle de qualidade parece ser de igual ou maior importância para uma adaptação mitocondrial adequada. Um desses mecanismos de controle de qualidade mitocondrial envolve a remoção de mitocôndrias danificadas/envelhecidas via autofagia mitocondrial (mitofagia). Contudo, os mecanismos envolvidos na mitofagia induzida pelo EFA são pouco conhecidos. Considerando o papel da adaptação mitocondrial sobre os efeitos benéficos do EFA, realizamos um estudo exploratório para buscar novos mecanismos envolvidos neste processo. Para isso, utilizamos uma abordagem proteômica direcionada à fração mitocondrial muscular de camundongos submetidos a uma única sessão de EFA. Num primeiro estudo, utilizamos os resultados de proteômica para procurar por proteínas envolvidas na ativação da mitofagia durante o EFA. A partir desse estudo, verificamos que uma sessão de EFA de fato induz sinais de mitofagia na musculatura esquelética. Além disso, propomos que as proteínas Phb2 e Mief2 podem acumular em mitocôndrias danificadas durante o EFA e colaborar para o recrutamento da maquinaria autofágica para a organela, auxiliando no controle de qualidade e adaptação mitocondrial induzidos pelo EFA. Em segundo estudo, tivemos como objetivo identificar nos resultados de proteômica possíveis reguladores de transcrição gênica envolvidos na adaptação mitocondrial induzida pelo EFA. Dessa maneira, identificamos que a proteína mitocondrial Spryd4, cuja função não havia sido estudada até então, parece aumentar na fração mitocondrial muscular durante o EFA. Observamos ainda que a expressão gênica muscular de Spryd4 diminui em camundongos idosos ou com distrofia muscular, aumenta em animais saudáveis após treinamento físico aeróbio e também parece aumentar em humanos treinados. In vitro, observamos que a atenuação da expressão de Spryd4 em miotubos primários promove disfunção mitocondrial, associada à diminuição da expressão de genes de complexos mitocondriais e envolvidos no transporte e metabolismo de lipídeos, além de promover atrofia de miotubos. Num contexto geral, a análise do proteoma mitocondrial muscular após uma sessão de EFA nos permitiu identificar proteínas que parecem estar envolvidas em adaptações mitocondriais, em especial, em mecanismos de mitofagia e controle do fluxo de substratos energéticosIncreased oxidative capacity induced by regular aerobic exercise (AE) is considered a major factor in health. Skeletal muscle is one of the most compromised tissues during exercise and has remarkable metabolic and structural plasticity upon mechanical stimuli. Muscles are rich in mitochondria and heavily reliant on oxidative phosphorylation for energy production. Thus, increased aerobic capacity induced by regular AE occurs largely due to mitochondrial adaptations. Many studies have shown that AE is able to induce mitochondrial biogenesis, and the transcription coactivator PGC-1?1 is known to coordinated gene expression both in nuclei and mitochondria. However, muscle-specific PGC-1?1 knockout mice still display major mitochondrial remodeling after AE training, supporting the existence of unknown mechanisms of AE-induced mitochondrial adaptations. Although making new mitochondria is crucial, the maintenance of a healthy pool of this organelle through mechanisms of quality control seems to be of equal or greater importance during mitochondrial adaptation. One mechanism for mitochondrial quality control comprises the removal of damaged/aged mitochondria via autophagy (mitophagy). Nonetheless, the mechanisms of AE-induced mitophagy are poorly understood. Given the importance of mitochondrial adaptation to the health benefits of AE, we conducted an exploratory study to uncover new mechanisms underlying this process. For this, we performed a proteomic analysis in the skeletal muscle mitochondria-enriched fractions of mice submitted to a single bout of AE. In a first study, we have used these proteomics data to seek for proteins that might be involved in AE-induced mitophagy. On this matter, we confirmed that a single bout of AE in mice increases skeletal muscle mitophagy signaling. Additionally, we suggest that Phb2 and Mief2 accumulate in damaged mitochondria in skeletal muscle during AE and might assist in the recruitment of the autophagic machinery to the organelle, thus aiding to mitochondrial quality control and AE-induced mitochondrial adaptation. In a second study, we have used the same proteomics data to identify transcriptional regulators that might have a role in AE-induced mitochondrial adaptation. Thereby, we have found that the mitochondrial protein Spryd4, whose function was so far unknown, seems to increase in the skeletal muscle mitochondria-enriched fractions following AE. Here we show that skeletal muscle Spryd4 gene expression decreases in aged and dystrophic mice, increases in healthy trained animals and also seems to increase in trained humans. In vitro, we have seen that Spryd4 loss of function in primary myotubes promotes mitochondrial dysfunction, decreases expression of genes involved in mitochondrial complex function, as in fatty acid oxidation and transport. Indeed, Spryd4 loss of function promoted myotube atrophy. Taken together, by analyzing the skeletal muscle mitochondrial proteome after a single bout of AE in mice, we have identified proteins that might participate in AE-induced mitophagy and substrate metabolism, and thus in skeletal muscle adaptation to A

Role of the lysosomal/autophagic proteolytic system in skeletal muscle of heart failure animals

INTRODUÇÃO: A atrofia muscular induzida pela insuficiência cardíaca (IC) está associada à intolerância ao exercício físico e ao mau prognóstico. Compreender os mecanismos moleculares envolvidos nessa atrofia pode contribuir para o desenvolvimento de estratégias terapêuticas para prevenir ou tratar tal condição. Tem sido demonstrado que o sistema proteolítico lisossomal/autofágico é um importante mecanismo de manutenção da massa muscular. Entretanto, o papel desse sistema no desenvolvimento da miopatia esquelética induzida pela IC ainda não havia sido abordado. Assim, o objetivo do presente estudo foi avaliar a atuação de componentes do sistema lisossomal/autofágico na musculatura esquelética de ratos submetidos ao infarto do miocárdio (IM). MÉTODOS: Cirurgias de IM e fictícia (Sham) foram realizadas em ratos Wistar, e doze semanas após os procedimentos cirúrgicos foram avaliados parâmetros ecocardiográficos, tolerância ao exercício físico e histologia dos tecidos cardíaco e muscular esquelético. Componentes do sistema proteolítico lisossomal/autofágico na musculatura esquelética foram avaliados por meio de expressão gênica (qRT-PCR) e proteica (Western Blotting) e atividade enzimática. RESULTADOS: Ratos IM apresentaram intolerância ao esforço físico, disfunção e dilatação ventricular esquerda e edema pulmonar, o que evidencia a presença de IC. Foi observado aumento da expressão gênica de GABARAPL1, ATG7, BNIP3, CTSL1 e LAMP2 no músculo glicolítico plantar, enquanto nenhuma alteração foi observada no músculo oxidativo sóleo, embora ambos os músculos tenham apresentado atrofia. Ainda, o IM promoveu no músculo plantar aumento da expressão proteica de Bnip3 e Fis1, maior atividade enzimática da Catepsina L e maior acúmulo de hidroperóxidos lipídicos. CONCLUSÕES: Nossos resultados evidenciam demonstram aumento da transcrição de genes relacionados à autofagia na atrofia do músculo plantar induzida por IM, mas não na atrofia do músculo sóleo. Assim, genes autofágicos são regulados de forma diferenciada em músculos atróficos compostos por diferentes tipos de fibras e características metabólicas. Ainda, alterações em componentes do sistema lisossomal/autofágico no músculo plantar indicam aumento da autofagia de mitocôndrias (mitofagia), o que parece ter contribuído para a atrofia deste músculo e para a intolerância ao exercício físico induzida pela ICINTRODUCTION: Heart failure (HF)-induced skeletal muscle atrophy is often associated to exercise intolerance and poor prognosis. Better understanding the molecular mechanisms underlying HF-induced muscle atrophy may contribute to the development of pharmacological strategies to prevent or treat such condition. It has been shown that autophagy-lysosome system is an important mechanism for maintenance of muscle mass. However, its role in HF-induced myopathy has not been addressed yet. Therefore, the aim of present study was to evaluate the relative role of the main autophagy-related genes in myocardial infarction (MI)-induced muscle atrophy in rats. METHODS: Wistar rats underwent MI or sham surgeries, and after 12 weeks were submitted to echocardiography, exercise tolerance and histology evaluations. Lysosomal/autophagic proteolytic system components were depicted in skeletal muscle by gene (qRT-PCR) and protein (Western Blotting) expression analysis, and enzymatic activity. RESULTS: MI rats displayed exercise intolerance, left ventricle dysfunction and dilation suggesting the presence of HF. The key finding of the present study is that upregulation of autophagy-related genes (GABARAPL1, ATG7, BNIP3, CTSL1 and LAMP2) was observed only in plantaris while muscle atrophy was depicted in both soleus and plantaris muscles. Furthermore, MI induced higher Bnip3 and Fis1 protein expression, and increased cathepsin L activity and lipid hydroperoxides levels in plantaris muscle. CONCLUSIONS: Altogether our results provide evidence for transcriptional overexpression of autophagy-related genes in MI-induced plantaris atrophy but not soleus atrophy. Therefore, autophagy-related genes are differentially regulated in atrophic muscles comprising different fiber-types and metabolic characteristics. Moreover, changes in lysosomal/autophagic system components in the plantaris muscle indicate increased mitochondrial autophagy (mitophagy), which seems to have contributed to HF-induced plantaris atrophy and exercise intoleranc

β2-Adrenergic Signaling Modulates Mitochondrial Function and Morphology in Skeletal Muscle in Response to Aerobic Exercise

The molecular mechanisms underlying skeletal muscle mitochondrial adaptations induced by aerobic exercise (AE) are not fully understood. We have previously shown that AE induces mitochondrial adaptations in cardiac muscle, mediated by sympathetic stimulation. Since direct sympathetic innervation of neuromuscular junctions influences skeletal muscle homeostasis, we tested the hypothesis that β2-adrenergic receptor (β2-AR)-mediated sympathetic activation induces mitochondrial adaptations to AE in skeletal muscle. Male FVB mice were subjected to a single bout of AE on a treadmill (80% Vmax, 60 min) under β2-AR blockade with ICI 118,551 (ICI) or vehicle, and parameters of mitochondrial function and morphology/dynamics were evaluated. An acute bout of AE significantly increased maximal mitochondrial respiration in tibialis anterior (TA) isolated fiber bundles, which was prevented by β2-AR blockade. This increased mitochondrial function after AE was accompanied by a change in mitochondrial morphology towards fusion, associated with increased Mfn1 protein expression and activity. β2-AR blockade fully prevented the increase in Mfn1 activity and reduced mitochondrial elongation. To determine the mechanisms involved in mitochondrial modulation by β2-AR activation in skeletal muscle during AE, we used C2C12 myotubes, treated with the non-selective β-AR agonist isoproterenol (ISO) in the presence of the specific β2-AR antagonist ICI or during protein kinase A (PKA) and Gαi protein blockade. Our in vitro data show that β-AR activation significantly increases mitochondrial respiration in myotubes, and this response was dependent on β2-AR activation through a Gαs-PKA signaling cascade. In conclusion, we provide evidence for AE-induced β2-AR activation as a major mechanism leading to alterations in mitochondria function and morphology/dynamics. β2-AR signaling is thus a key-signaling pathway that contributes to skeletal muscle plasticity in response to exercise

Resistance training-induced changes in integrated myofibrillar protein synthesis are related to hypertrophy only after attenuation of muscle damage

Key points Skeletal muscle hypertrophy is one of the main outcomes from resistance training (RT), but how it is modulated throughout training is still unknown. We show that changes in myofibrillar protein synthesis (MyoPS) after an initial resistance exercise (RE) bout in the first week of RT (T1) were greater than those seen post-RE at the third (T2) and tenth week (T3) of RT, with values being similar at T2 and T3. Muscle damage (Z-band streaming) was the highest during post-RE recovery at T1, lower at T2 and minimal at T3. When muscle damage was the highest, so was the integrated MyoPS (at T1), but neither were related to hypertrophy; however, integrated MyoPS at T2 and T3 were correlated with hypertrophy. We conclude that muscle hypertrophy is the result of accumulated intermittent increases in MyoPS mainly after a progressive attenuation of muscle damage. AbstractSkeletal muscle hypertrophy is one of the main outcomes of resistance training (RT), but how hypertrophy is modulated and the mechanisms regulating it are still unknown. To investigate how muscle hypertrophy is modulated through RT, we measured day-to-day integrated myofibrillar protein synthesis (MyoPS) using deuterium oxide and assessed muscle damage at the beginning (T1), at 3weeks (T2) and at 10weeks of RT (T3). Ten young men (27(1)years, mean (SEM)) had muscle biopsies (vastus lateralis) taken to measure integrated MyoPS and muscle damage (Z-band streaming and indirect parameters) before, and 24h and 48h post resistance exercise (post-RE) at T1, T2 and T3. Fibre cross-sectional area (fCSA) was evaluated using biopsies at T1, T2 and T3. Increases in fCSA were observed only at T3 (P=0.017). Changes in MyoPS post-RE at T1, T2 and T3 were greater at T1 (

Impaired oxygen-sensitive regulation of mitochondrial biogenesis within the von Hippel-Lindau syndrome

Mitochondria are the main consumers of oxygen within the cell. How mitochondria sense oxygen levels remains unknown. Here we show an oxygen-sensitive regulation of TFAM, an activator of mitochondrial transcription and replication, whose alteration is linked to tumours arising in the von Hippel–Lindau syndrome. TFAM is hydroxylated by EGLN3 and subsequently bound by the von Hippel–Lindau tumour-suppressor protein, which stabilizes TFAM by preventing mitochondrial proteolysis. Cells lacking wild-type VHL or in which EGLN3 is inactivated have reduced mitochondrial mass. Tumorigenic VHL variants leading to different clinical manifestations fail to bind hydroxylated TFAM. In contrast, cells harbouring the Chuvash polycythaemia VHL(R200W) mutation, involved in hypoxia-sensing disorders without tumour development, are capable of binding hydroxylated TFAM. Accordingly, VHL-related tumours, such as pheochromocytoma and renal cell carcinoma cells, display low mitochondrial content, suggesting that impaired mitochondrial biogenesis is linked to VHL tumorigenesis. Finally, inhibiting proteolysis by targeting LONP1 increases mitochondrial content in VHL-deficient cells and sensitizes therapy-resistant tumours to sorafenib treatment. Our results offer pharmacological avenues to sensitize therapy-resistant VHL tumours by focusing on the mitochondria

Erratum to: Guidelines for the use and interpretation of assays for monitoring autophagy (3rd edition) (Autophagy, 12, 1, 1-222, 10.1080/15548627.2015.1100356

non present