2.1 Cell culture, reagents, and antibodies

Mouse skeletal muscle C2C12 myoblasts were cultivated in growth medium consisting of high-glucose Dulbecco's modified Eagle's medium (DMEM; Gibco, Carlsbad, CA) supplemented with 10% fetal bovine serum (Batch Number 1693362), 1% non-essential amino acids (Gibco), and 20 mM n-2-hydroxyethylpiperazine-n-2-ethane sulfonic acid (HEPES; Gibco). Upon reaching 80–90% confluence, cells were seeded in 12-well CellBIND plates (Coring Life Science, Lowell, CA) or staining slide flasks (Nunc Lab-Tek Flask on Slide; Thermo Fisher Scientific, Waltham, MA) at a density of 100,000 cells/well or 240,000 cells/slide flasks, respectively. Following seeding, cells were allowed to grow for 24 hr in growth medium. Then, C2C12 myoblasts were differentiated into myotubes for 5 days in high-glucose DMEM supplemented with 2% horse serum (Gibco), 1% non-essential amino acids (Gibco), and 20 mM HEPES (Gibco).

2.2 In silico analysis

TargetScanMouse, miRanda, and microT-CDS algorithms were used to predict the targets of miRNA-204-5p. Predicted targets were only considered when they were predicted by at least two of the databases. In addition, all predictions present at least a 7mer site-matching, meaning that the entire seed sequence of miRNA-204-5p matches the 3′- untranslated region (3′-UTR) sequence of the gene of interest.

2.3 C2C12 transfection

At Day 5 of differentiation, C2C12 myotubes were transfected with either a specific miRCURY LNA™ miRNA inhibitor targeting miRNA-204-5p (Exiqon A/S, Vedbæk, Denmark), or a specific locked nucleic acid (LNA) inhibitor, was used as a negative control. This control LNA (sequence: TAACACGTCTATACGCCCA) does not target any known mature miRNA.

Transfection was performed using lipofectamine RNAiMAX (Invitrogen, Carlsbad), according to the manufacturer's instructions. Shortly, lipofectamine complexes were stabilized in OptiMEM (Gibco) for 5 min and incubated with the LNAs, diluted to 500 nM in OptiMEM, for 20 min. Finally, the lipofectamine/LNA complexes were diluted 1:5 in differentiation media (Dahlmans et al., 2017).

2.4 RNA preparation and gene expression analysis in C2C12 cells

Cells were washed with 1 ml cold 1X phosphate-buffered saline (PBS) and harvested in 700 µl TRIzol reagent (Invitrogen) and kept at −80^oC for subsequent analyses. RNeasy Mini Kits (Qiagen, Venlo, The Netherlands) were used to extract RNA. RNA quantity and quality were measured using a nanodrop microvolume spectrophotometer (ND-1000; NanoDrop Technologies, Wilmington, DE) and complementary DNA (cDNA) was synthesized using the High-Capacity RNA-to-cDNA Kit (Applied Biosystems) according to manufacturer's guidelines. Quantitative polymerase chain reaction (qPCR) was performed using the SensiMix SYBR Hi-ROX Kit (Bioline, London, UK) and specific primer sets (Sigma-Aldrich, St. Louis, MI) to quantify the abundance of mRNAs of interest. The qPCR analyses were performed on the CFX384 Touch™ Real-Time PCR Detection System (Bio-Rad, Hercules, CA).

2.5 Mitochondrial DNA copy number quantification

For the determination of mitochondrial DNA (mtDNA) copy number, DNA was isolated at 24, 36, and 48 hr posttransfection using the DNeasy Blood & Tissue Kit (Qiagen). DNA was quantified and the integrity was checked by spectrophotometry using the Nanodrop. Relative amounts of nuclear and mtDNA were quantified by qPCR, in which nuclear DNA was represented by the UCP2 gene and mtDNA by the COX2 gene. qPCR was performed on the ABI Prism 7900HT Real-Time PCR System (Applied Biosystems, Foster City, CA). MtDNA copy number was calculated using the ΔC_t method.

2.6 Luciferase reporter assay

C2C12 cells were cultured in DMEM (4.5 g/L d-glucose) supplemented with 10% fetal bovine serum, 2% HEPES, and 1% minimum essential medium non-essential amino acids solution and seeded in 24-well plates at a density of 50,000 cells/well. The next day, cells were transfected with hsa-miRNA-204-5p or Neg control #1 (Ambion; Life Technologies, Waltham) precursor molecules and cotransfected with the LightSwitch_PPARGC1A_3′UTR vector (Active Motif, Carlsbad) using Lipofectamine 2000 (Invitrogen, Waltham). After 24 hr, the luciferase activity was determined using the LightSwitch Luciferase Assay Reagent (SwitchGear Genomics, Carlsbad) according to the manufacturer's instructions using a GLOMAX Microplate Luminometer (Promega Corporation, Madison, WI).

2.7 Microarray analysis

Purified RNA was labeled with the Ambion WT Expression Kit (Carlsbad) and hybridized to an Affymetrix Mouse Gene 1.1 ST array plate (Affymetrix, Santa Clara, CA). Hybridization, washing, and scanning were carried out on an Affymetrix GeneTitan platform according to the manufacturer's instructions. Normalized expression estimates were obtained from the raw intensity values applying the robust multiarray analysis preprocessing algorithm available in the Bioconductor library affyPLM with default settings (Bolstad, Irizarry, Astrand, & Speed, 2003; Irizarry et al., 2003). Probe sets were defined according to Dai et al. (2005). In this method, probes are assigned to Entrez IDs as a unique gene identifier. In this study, probes were reorganized based on the Entrez Gene database, build 37, Version 1 (remapped CDF v22). q values were calculated using an intensity-based moderated T-statistic (Sartor et al., 2006). Genes were defined as significantly changed when q < .05.

2.8 Protein extraction and western blot analysis in C2C12 muscle cells

Cells were washed with 1 ml cold 1X PBS and scraped in 150 µl Bio-Plex cell lysis buffer (Bio-Rad), and processed according to the manufacturer's instruction. Protein loading for each sample was first determined using InstantBlue Coomassie (Expedeon, San Diego, CA). Equal amounts of protein were loaded in precast sodium dodecyl sulfate-polyacrylamide gel electrophoresis (Mini TGX AnyKD or Criterion TGX AnykD; Bio-Rad). Next, LC3B-I and LC3B-II were detected using an antibody directed against LC3B, diluted 1:1000 (L7543; Sigma-Aldrich). Furthermore, an antibody directed against β-actin was diluted 1:25,000 (A5316; Sigma-Aldrich), and was used as a loading control. Finally, membranes were quantified at the appropriate wavelengths using an Odyssey CLx Imaging System (Li-COR, Lincoln, NE).

2.9 Live cell imaging in C2C12 cells

C2C12 myoblasts were seeded in 12-well CellBIND plates (Corning) at 100,000 cells/well and allowed to settle overnight in the growth medium. Then, the medium was replaced to differentiation medium and cells were transfected as previously described. Continuous cell monitoring was performed for 10 days using the IncuCyte ZOOM (Essen Bioscience, Ltd., Hertfordshire, UK). The differentiation medium was replaced every 48 hr to maintain the cells for the duration of the experiments.

2.10 Immunocytochemistry in C2C12 cells

C2C12 myoblasts were seeded in slide flasks (Nunc Lab-Tek Flask on Slide; Thermo Fisher Scientific) at 240,000 cells/flask and differentiated for 5 days. Then, myotubes were transfected and fixated 48 hr posttransfection. To fix the cells, myotubes were washed three times in PBS and incubated for 1 hr in 3.7% formaldehyde at room temperature. Finally, fixed myotubes were washed three times in PBS and stored in PBS at 4°C until immunocytochemistry was performed. Before staining, slides were rinsed for 5 min in PBS and directly incubated with primary antibodies diluted in 0.05% Tween-20 in PBS. Mitochondria were stained by an anti-OxPhos antibody cocktail (MS604; MitoSciences, Eugene, OR), targeting structural subunits of all OxPhos complexes. Autophagosomes were visualized by using an anti-LC3B antibody (L7543; Sigma-Aldrich). Image acquisition was performed using a Nikon Eclipse E800 fluorescent microscope equipped with ×40 oil immersion objective (Nikon Instruments, Amsterdam, The Netherlands) or a Leica TCS SP8 confocal microscope equipped with a ×63 1.40NA oil immersion objective (Leica, Amsterdam). The confocal images were processed using deconvolution software (Huygens Professional; Scientific Volume Imaging B.V., Hilversum, The Netherlands).

2.11 Subject selection and human muscle biopsies collection

The subjects included in this study participated in previous studies (Phielix, Meex, Moonen-Kornips, Hesselink, & Schrauwen, 2010; Phielix et al., 2012; Vosselman et al., 2015; van de Weijer et al., 2015) that were approved by the institutional medical ethics committee, registered at ClinicalTrials.gov (NCT00943059 and NCT01298375) and in the Dutch trial register (NL1888) and for which all participants provided their written informed consent in accordance with the declaration of Helsinki. From these studies, we selected four groups of male, weight-stable individuals for the analysis of miRNA-204-5p expression in skeletal muscle and its relation to parameters for in vivo oxidative capacity. These four groups included: (a) Type 2 diabetic patients (n = 12); (b) overweight/obese nondiabetic subjects (n = 12); (c) young lean individuals (n = 12), and (d) young endurance-trained athletes (n = 12). The primary selection was based on the availability of muscle material and the presence of reliable data for in vivo oxidative capacity (maximal aerobic capacity [VO₂ max] and phosphocreatine [PCr] recovery rate). Second, subjects were also selected with the intention to create age- and body mass index-matched groups (i.e., Group 1 vs. Group 2 and Group 3 vs. Group 4).

All Type 2 diabetes patients were on metformin treatment and the use of statins was permitted. Obese nondiabetic individuals were considered healthy, that is, they did not use medication, did not present any pathology (hypertension, cardiovascular disorders, and liver dysfunction), and did not have any first-degree relatives with Type 2 diabetes.

Lean sedentary (LS) subjects were included if their VO₂ max was below 45 ml⁻¹·min⁻¹·kg and did not participate in more than 1 hr of organized exercise per week for the previous 2 years. Endurance-trained athletes were enrolled in the study if their VO₂ max was higher than 55 ml⁻¹·min⁻¹·kg and if they participated in endurance training at least three times per week for the last 2 years.

All biopsies were collected after an overnight (≥10 hr) fast and before any intervention. Subjects were instructed to avoid (strenuous) physical exercise in the 3-day period preceding the muscle biopsy.

2.12 Subject characterization

All subjects included in this study were thoroughly phenotyped in term of body composition and aerobic capacity. Body composition was determined either via dual X-ray absorptiometry (Discovery A; Hologic, Bedford, MA) or hydrostatic weighing (Siri, 1993). Maximal aerobic capacity was determined through an incremental cycling test until exhaustion, as described previously (Kuipers, Verstappen, Keizer, Geurten, & van Kranenburg, 1985). In vivo mitochondrial function was assessed via quantification of PCr resynthesis rates using a 31P magnetic resonance spectrometry approach on a 3 T whole-body scanner (Achieve 3T-X; Philips Healthcare, The Netherlands), as previously described (Lindeboom et al., 2014).

2.13 MiRNA quantitative PCR in muscle biopsies

A 10–15 mg piece of frozen muscle tissue was homogenized in 700 µl of TRIzol with an Ultra-Turrax (IKA, Staufen, Germany) for 1 min at 17,000 rpm. RNA isolation was then performed using a miRNeasy Mini Kit (Qiagen) according to the manufacturer's instructions. The yield was improved by reloading the final eluate onto the column membrane twice. RNA concentrations were measured using a microvolume spectrophotometer (Nanodrop), whereas RNA quality was determined using a Bioanalyzer System (Agilent Technologies, Santa Clara, CA). Then, cDNA synthesis was performed using the Universal cDNA Synthesis Kit II (Exiqon) according to the manufacturer's protocol. Finally, cDNA samples were analyzed using predesigned 384-well Pick-&-Mix microRNA PCR Panel plates (Exiqon), according to the manufacturer's guidelines using a CFX384 Touch Real-time PCR Detection System (Bio-Rad). Relative miRNA expression levels were determined using the ΔΔC_t method. Synthetic UniSP6 spike-in control was used to monitor the cDNA synthesis reaction, that is, as a positive control of the reverse transcription. Furthermore, an interpolate calibrator was added to all qPCR plates to uniformly normalize C_t values across all the experiments.

2.14 Statistics analysis

All results are expressed as means ± standard deviation. Each set of in vitro data presented in this study is the result of three independently executed experiments, each of which includes three technical replicates (unless indicated otherwise in the figure legend). Comparisons between in vitro conditions were performed by unpaired two-tailed Student's t test. Comparisons over time were performed by two-way analysis of variance (ANOVA). p < .05 was considered statistically significant.

Differences between the various human subject groups were assessed via one-way ANOVA with Tukey's multiple comparisons test. Pearson correlation analysis was used to correlate miRNA-204-5p expression in skeletal muscle to in vivo parameters of oxidative capacity.

3.1 miRNA-204-5p silencing in C2C12 myotubes increases PGC-1α gene expression

We previously silenced 19 individual candidate miRNAs, identified in a large miRNA-silencing screen (Dahlmans et al., 2017), and subsequently measured 27 genes involved in mitochondrial function (Dahlmans et al., 2019). Interestingly, the silencing of miRNA-204-5p showed a pronounced induction of the expression of PGC-1α, a well-known regulator of mitochondrial biogenesis, both when silenced for 24 (2.43-fold; p < .05) and 48 hr (3.71-fold; p < .01; Figure 1). Subsequent in silico analysis by TargetScan and miRanda revealed a specific sequence in the 3′-UTR of PGC-1α as a predicted target to the seed region of miRNA-204-5p (Figure 1a). In addition, both miRNA-204-5p and the binding site in the 3′-UTR of PGC-1α were conserved over many different invertebrates as well as vertebrate species including humans, but not worm (Figure 1a). Moreover, activity assays using a luciferase reporter construct harboring the PGC-1α 3′-UTR revealed that increasing concentrations of pre-miRNA-204-5p significantly and dose-dependently reduced the luciferase reporter signal, indicating a functional interaction between miRNA-204-5p and the 3′-UTR of PGC-1α (Figure 1b).

To address the consequences of the increase in PGC-1α expression (Figure 1c), we next assessed citrate synthase activity as well as mtDNA copy number as markers for mitochondrial density. In line with the elevated PGC-1α expression, citrate synthase activity (Figure 1d) showed a strong tendency to be increased after 24 hr miRNA-204-5p silencing (25% increase; p = .06), whereas the difference did not reach statistical significance at 48 hr. MtDNA copy number was significantly increased (46% increase; p < .05) 36 hr posttransfection, but not after 24 or 48 hr miRNA-204-5p silencing (Figure 1e). Together, these results indicate a (transient) increase in mitochondrial content upon miRNA-204-5p silencing, which prompted us to further analyze the role of miRNA-204-5p in regulating mitochondrial metabolism.

3.2 miRNA-204-5p silencing induces morphological aberrations in C2C12 myotubes

To investigate if the silencing of miRNA-204-5p also resulted in morphological changes that could reveal enhanced mitochondrial density, we next studied the effect of miRNA-204-5p silencing on C2C12 myotube development and continuously monitored the transfected C2C12 myotubes for 72 hr after transfection. Interestingly, myotubes transfected with anti-miRNA-204-5p displayed morphological changes that were most apparent 48 hr posttransfection. Thus, whereas nontransfected and Negative Control A transfected C2C12 myotubes displayed a normal morphology and similar appearance as control cells (Figure 2a–e) 48 hr posttransfection, (i.e., at Day 7 of differentiation) myotubes transfected with anti-miRNA-204-5p showed large round anomalous structures within the myotubes (Figure 2f–j).

Strikingly, when undifferentiated C2C12 muscle cells were transfected with anti-miRNA-204-5p and subsequently underwent differentiation, the aberrant structures did not appear before Day 5 of differentiation (Figure 3). In other words, C2C12 muscle cells transfected with Negative Control A or anti-miRNA-204-5p in the myoblasts stage, displayed similar and normal morphology during the first 4 days of subsequent differentiation (Figure 3). Again, although the morphological abnormalities started to appear at Day 5 of differentiation, the irregular cellular morphology was most apparent at Day 7 of differentiation (Figure 3h), comparable to the changes seen after silencing miRNA-204-5p in already differentiated C2C12 myotubes.

3.3 Silencing of miRNA-204-5p affects markers for autophagy/mitophagy

We next hypothesized that the abnormal phenotype of the C2C12 myotubes upon miRNA-204-5p silencing could possibly be explained by increased autophagic activity, especially since microtubule-associated protein 1A/1B-LC3B, a major player in autophagosome formation, is another predicted target (Figure 4a) of miRNA-204-5p as shown previously in renal cell carcinoma (Mikhaylova et al., 2012). To study whether the morphological abnormalities that we observed in the C2C12 myotubes could be related to autophagy, we first performed a microarray analysis 24 hr posttransfection and focused on the expression of several autophagy-related genes. Indeed, the miRNA-204-5p predicted target LC3B, as well as autophagosome and lysosome fuser VAMP8 and lysosomal cysteine protease inhibitor cystatin B (CSTB), were significantly increased following anti-miRNA-204-5p treatment (Figure 4b). A similar expression pattern was observed for the autophagy markers GABARAPL1 and SQSTM1 (Figure 4b), although these changes did not reach statistical significance. Interestingly, however, mitophagy markers PARK2, BNIP3, BNIP3L, and FUNDC1 appeared to be decreased after miRNA-204-5p lowering, although this was only statistically significant for FUNDC1 (Figure 4b).

Next, to investigate if the induction of autophagy markers was translated to the protein level, we quantified the abundance of LC3B-I and LC3B-II protein 12, 24, 36, 48, and 72 hr posttransfection. Despite the apparent induction of several autophagy-related genes and the aberrant phenotype of the cells, 48 hr posttransfection with anti-miRNA-204-5p (as displayed in Figure 2), we could not detect changes in protein abundance of LC3B-I or LC3B-II after silencing miRNA-204-5p (Figure 4c). However, since we previously demonstrated that the morphological phenotype only occurs in fully differentiated C2C12 myotubes, and not myoblasts, changes in LC3B abundance might have been masked by the presence of undifferentiated myoblasts in our cell cultures. To circumvent this problem, we finally performed immunocytochemistry with an antibody against LC3B and investigated LC3B in miRNA-204-5p silenced C2C12 myotubes. Indeed, while C2C12 myotubes transfected with Negative Control A displayed a diffuse, ubiquitous LC3B expression (Figure 5a), miRNA-204-5p silencing induced a typical punctuated staining of LC3B, 48 hr posttransfection (Figure 5b). The observed LC3B staining was similar to the pattern observed in C2C12 myotubes transfected with Negative Control A and subsequently treated with chloroquine, which is known to induce the accumulation of LC3B-positive autophagosomes by inhibiting their clearance (Figure 5c). Finally, we performed double staining for LC3B and OxPhos, as a marker for mitochondria, in C2C12 myotubes, 48 hr posttransfection with either Negative Control A or anti-miRNA-204-5p. Interestingly, whereas OxPhos displayed a diffuse homogenous staining in the Negative Control A transfected cells, we observed a punctuated OxPhos localization in the anti-miRNA-204-5p transfected cells that were similar to the LC3B staining pattern. Furthermore, the merged images of OxPhos and LC3B demonstrated the colocalization of both mitochondria and the autophagosomal marker LC3B (Figure 6).

3.4 miRNA-204-5p expression correlates to in vivo mitochondrial function in human skeletal muscle

To test whether these findings are relevant in human physiology, we then selected (from previous human clinical trials performed in our facilities [Phielix et al., 2010; Phielix et al., 2012; van de Weijer et al., 2015; Vosselman et al., 2015]) four subject groups known to be characterized by different mitochondrial abundance and oxidative capacity, including Type 2 diabetes patients (Type 2 diabetes mellitus [T2DM]), obese nondiabetic subjects (O), LS individuals, and endurance-trained athletes (A) and investigated miRNA-204-5p expression in skeletal muscle biopsies. Also, VO₂ max and PCr recovery rates were determined, although the latter could not be assessed in the entire cohort (n = 38). The characteristics of the subjects included for the current study are displayed in Table 1. VO₂ max and PCr recovery were highest in endurance-trained athletes and lowest in patients with T2DM (Table 1).

Interestingly, the expression of miRNA-204-5p in skeletal muscle was different between the Type 2 diabetic individuals and endurance-trained athletes as assessed by one-way ANOVA with Tukey's post hoc correction for multiple testing. Thus, the expression of miRNA-204-5p was 1.85-fold (p = .008) higher in Type 2 diabetes patients with a low mitochondrial oxidative capacity when compared to the endurance-trained athletes with an optimal mitochondrial oxidative capacity (Figure 7a). In addition, miRNA-204-5p expression negatively correlated with VO₂ max (r = −.38, p = .011; Figure 7b) and positively correlated with PCr recovery rates (r = .37, p = .023; Figure 7c). Collectively, these collective results indicate that low miRNA-204-5p expression is associated with high in vivo mitochondrial oxidative capacity in humans, that is, a high VO₂ max and a fast PCr recovery.