Myostatin Increases Smad2 Phosphorylation and Atrogin-1 Expression in Chick Embryonic Myotubes.

Skeletal muscle mass is an important trait in poultry meat production. In mammals, myostatin, a negative regulator of skeletal muscle growth, activates Smad transcription factors and induces the expression of atrogin-1 by regulating the Akt/FOXO pathway. Although the amino acid sequence of chicken myostatin is known to be completely identical to its mammalian counterpart, previous studies in chicken skeletal muscles have implied that the physiological roles of chicken myostatin are different from those of mammals. Furthermore, it remains to be elucidated whether myostatin affects cellular signaling factors and atrogin-1 expression. In this study, using chick embryonic myotubes, we found that myostatin significantly increased the phosphorylation rate of Smad2 and mRNA levels of atrogin-1. No significant change was observed in the phosphorylation of Akt and FOXO1. These in vitro results suggest that the molecular mechanisms underlying myostatin-induced expression of atrogin-1 might be different between chickens and mammals. 2019, Japan Poultry Science Association.

Introduction

Skeletal muscle mass is an important trait in poultry meat production. Since it is controlled by a balance between protein synthesis and degradation, a number of studies have been carried out to clarify the mechanisms underlying protein metabolism in poultry skeletal muscle.

Numerous lines of evidence indicate that Akt-mediated signaling pathways play critical roles in regulating protein synthesis and proteolysis in muscle cells (Glass, 2005; Sandri, 2008, 2013; Schiaffino ; Sanchez ). For example, activation of the Akt/mTOR pathway stimulates protein synthesis. The phosphorylated Akt directly phosphorylates and inactivates FOXO, which is a major transcription factor of atrophy-related genes, atrogenes, such as atrogin-1 and MuRF-1 (Foletta ; Gumucio and Mendias, 2013). Atrogin-1 and MuRF-1, two muscle-specific E3 ubiquitin ligases, induce the degradation of myofibril proteins. Therefore, the activation of Akt-mediated pathways and expression of atrogenes have been generally examined to understand protein metabolism in skeletal muscle.

Myostatin, a member of the transforming growth factor-β (TGF-β) superfamily, has been demonstrated to inhibit muscle mass development in mammals (McPherron ; Huang ; Rodriguez ). For example, individual muscles of myostatin null mice weigh 2–3 times more than those of wild-type mice, and the increase in skeletal muscle mass appears to result from a combination of hyperplasia and hypertrophy (McPherron ). Naturally occurring mutation in the myostatin gene leads to a hypermuscular phenotype in humans, mice, dogs, sheep, and cattle (Rodriguez ). In addition, myostatin plays a fundamental role in regulating adult muscle growth and size (Rodriguez ).

Accumulating evidence from previous studies have revealed the manner in which myostatin affects skeletal muscle growth. For example, myostatin downregulates the Akt/mTOR pathway and inhibits protein synthesis in C2C12 myotubes and mammalian skeletal muscles (Taylor ; Welle ; Amirouche ; Morissette ; Lipina ). A recent in vitro study showed that high concentrations (2–3 µg/mL) of myostatin significantly inhibited the mTOR pathway and protein synthesis, whereas low concentrations (0.01–1 µg/mL) of myostatin significantly induced the phosphorylation of AMP-activated protein kinase (AMPK) and inhibited protein synthesis without affecting the mTOR pathway (Deng ). In addition to the inhibition of protein synthesis, myostatin promotes the transcription of atrogin-1 by regulating Smads and the Akt/FOXO pathway (Gumucio and Mendias, 2013; Lokireddy ; McFarlane ). Smads are transcription factors that are phosphorylated after myostatin binds to its receptors (Huang ; Rodriguez ). A previous in vivo study reported that Smad3 was sufficient to induce an increase in atrogin-1 promoter activity in murine skeletal muscle that was co-transfected with Smad3 and atrogin-1 promoter (Goodman ). However, several in vitro and in vivo studies have shown that myostatin inhibits protein synthesis and the Akt/mTOR pathway without affecting protein degradation and expression of atrogin-1 and MuRF-1 (Taylor ; Welle ; Amirouche ). Collectively, results suggest that myostatin inhibits skeletal muscle growth mainly by downregulating Akt phosphorylation in mammals.

The amino acid sequence of mature myostatin is identical among humans, mice, rats, pigs, dogs, chickens, and turkeys (Huang ). However, previous studies have suggested that the roles of myostatin in skeletal muscles differ between mammals and chickens. For example, knockdown of the myostatin gene by RNA interference increased body, but not carcass, weight in chickens (Bhattacharya ), and myostatin expression was not altered in lines of poultry exhibiting myofiber hyper- and hypoplasia (Mott and Ivarie, 2002). In contrast to the results from previous studies on mammalian skeletal muscles which showed that myostatin expression increased due to food deprivation or restriction (Allen ; Zhao ), myostatin mRNA levels decreased due to fasting in chicken skeletal muscles (Guernec ; Saneyasu ). Furthermore, it remains to be elucidated as to how myostatin affects the cellular signaling factors and expression of atrogenes in chicken skeletal muscle. To clarify the mechanism underlying species-specific roles of myostatin in chicken skeletal muscle, we investigated the effects of myostatin on the mRNA and protein levels of protein metabolism-related factors in chick embryonic myotubes.

Materials and Methods

Cell Culture

Breast muscles dissected from 14-day-old chick embryos were minced using surgical scissors and digested with HBSS (+) (Nacalai Tesque, Inc., Kyoto, Japan) containing 0.2% collagenase (Worthington Biochemical Corp., Lakewood, NJ, USA) for 20 min at 37°C. The cells were collected by centrifugation and resuspended in DMEM (Nacalai Tesque, Inc., Kyoto, Japan) supplemented with 15% serum (Fetal Clone III, GE Healthcare Bio-Sciences AB, Uppsala, Sweden), 1× non-essential amino acid solution (Nacalai Tesque, Inc., Kyoto, Japan), and 1× gentamicin/amphotericin solution (Life Technologies, Carlsbad, CA, USA). The cell suspension was passed through a cell strainer to remove tissue debris and then transferred to an uncoated flask to allow attachment of fibroblasts. After 1 h, the unattached cells were transferred to another uncoated flask and this procedure was repeated 2–3 times. The unattached cells were counted and plated onto collagen I-coated 12-well plates at 1×105 cells/well. The cells were incubated in the medium described above at 37°C, with 5 % CO2 in a humidified chamber until the formation of myotubes. Myotubes were treated with or without 20nM recombinant human/rat/mouse myostatin (PeptroTech Inc., Rocky Hill, NJ, USA) for 2 h, in the absence or presence of serum.

Real-time PCR Analysis

The cells were washed with phosphate-buffered saline (PBS). Then, total RNA was extracted from the cells using Sepazol-RNA I (Nacalai Tesque, Inc., Kyoto, Japan). First-strand cDNA was synthesized from total RNA using Rever Tra Ace® qPCR RT Master Mix with gDNA Remover (Toyobo Co. Ltd, Osaka, Japan). The levels of mRNA were quantified for each primer (Table 1) using TB Green Premix Ex Taq II (Tli RNaseH Plus; Takara Bio Inc., Otsu, Japan) according to the supplier's recommendations, in an Applied Biosystems 7300 Real-Time PCR System (Applied Biosystems, Foster City, CA, USA). The expression levels of target genes were normalized to that of ribosomal protein S17 (RPS17).

Table 1.

Primer sequences used for real-time PCR analysis

Gene name	Forward primer	Reverse primer	Accession number
Atrogin-1	5′-cac ctt ggg aga agc ctt caa-3′	5′-ccg gga gtc cag gat agc a-3′	NM_001030956
FOXO1	5′-tct ggt cag gag gga aat gg-3′	5′-gct tgc agg cca ctt tga g-3′	NM_204328
MuRF-1	5′-tgg aga aga ttg agc aag gct at-3′	5′-gcg agg tgc tca aga ctg act-3′	XM_424369
Myostatin	5′-acc cac caa gat gtc ccc ta -3′	5′-acc cgc aac gat cta caa cc-3′	NM_001001461
RPS17	5′-gcg ggt gat cat cga gaa gt-3′	5′-gcg ctt gtt ggt gtg aag t-3′	NM_204217

FOXO, forkhead box class O; MuRF-1, muscle ring-finger protein 1; RPS17, ribosomal protein S17.

The primers of atrogin-1, FOXO1, MuRF-1, and RPS17 have been used in previous studies (Saneyasu , 2016, 2017).

Western Blot Analysis

Western blot analysis was performed as previously described by Saneyasu . Briefly, cells were rinsed with ice-cold PBS. Then, cells were scraped into 100 µL of lysis buffer. The cell lysates were ultrasonicated and centrifuged at 17,900×g for 15 min at 4°C. The supernatants were stored at −80°C. Protein concentrations were determined using the Pierce BCA Protein Assay Kit (Pierce Biotechnology, Rockford, IL, USA). The lysates (4 µg of protein) were subjected to sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and western blotting using HorizeBlot (ATTO Co., Tokyo, Japan), according to the manufacturer's instructions. Bands were detected by Chemi-Lumi one Super (Nacalai Tesque, Inc., Kyoto, Japan), visualized with the LumiCube (Liponics Inc., Tokyo, Japan), and quantified using the CS Analyzer software (ATTO Co., Tokyo, Japan). Anti-Akt (#9272), anti-phospho-Akt (pAkt) (Ser473) (#9271), anti-pAMPKα (Thr172) (#2531), anti-AMPKα (#2532), anti-FOXO1 (#9454), anti-pFOXO1 (Ser 256) (#9461), anti-pSmad2 (Ser465/467) / Smad3 (ser423/425) (#8828), anti-Smad2/3 (#8685), anti-β-actin (#4967), and horseradish peroxidase (HRP) -conjugated anti-rabbit IgG (#7074) were purchased from Cell Signaling Technology (Danvers, MA, USA). The species cross-reactivity is described in the manufacturer's data sheet. Additionally, we confirmed with the manufacturer that each antigen sequence for #2532, #8828, and #8685 has 88%, 100%, and 100% homology with that of chicken, respectively. When detecting pSmad2/3, FOXO1, and pFOXO1, antibodies were diluted with Can Get Signal (Toyobo Co. Ltd, Osaka, Japan).

Statistical Analysis

Data were analyzed using the Dunnett's test or t-test. All statistical analyses were performed using Excel 2013 (Microsoft, USA), with Statcel 3 add-in software (OMS, Tokyo, Japan).

Results

Myostatin significantly induced phosphorylation of Smad2 and expression of FOXO1 and atrogin-1 in chick embryonic myotubes cultured in the presence of serum, whereas no significant change was observed in the phosphorylation of Smad3, Akt, AMPK, and FOXO1, and in mRNA levels of MuRF-1 (Fig. 1). Although FOXO1 mRNA levels significantly increased, FOXO1 protein levels did not significantly change (Fig. 1). These results suggest that myostatin upregulates the expression of atrogin-1 and FOXO1 via Smad activation in an Akt/FOXO1 and AMPK pathway-independent manner.

Fig. 1.

(A) Effects of myostatin on the phosphorylation of Smad, Akt, FOXO1, and AMPK, (B) Effects of myostatin on the mRNA levels of FOXO1, atrogin-1, and MuRF-1, in the chick myotubes. The myotubes were treated with 15% serum-containing medium with or without (Con) 20nM myostatin (Mstn), for 2 h. Data are expressed as mean±standard error of the mean of five (A) and six (B) wells in each group. Student's t-test was used to analyze the differences. ** Significant with respect to control group (** P < 0.01).

The treatment with serum-free medium significantly increased mRNA levels of myostatin, atrogin-1, and MuRF-1 in chick myotubes (Fig. 2A). AMPK phosphorylation was significantly induced by serum-free treatment, whereas Akt phosphorylation was significantly inhibited (Fig. 2B). Unexpectedly, no significant change was observed in Smad2 and FOXO1 phosphorylation (Fig. 2B). In addition, FOXO1 mRNA levels were significantly decreased by serum-free treatment (Fig 2A), although no significant change was observed in its protein levels (Fig. 2B). All these findings suggest that serum-free treatment upregulates transcription of myostatin, atrogin-1, and MuRF-1, possibly via AMPK activation.

Fig. 2.

(A) Effects of serum-free conditions and myostatin treatment on the mRNA levels of myostatin, FOXO1, atrogin-1, and MuRF-1, (B) Effects of serum-free conditions and myostatin treatment on the phosphorylation of Smad, Akt, FOXO1, and AMPK, in the chick myotubes. The myotubes were treated with either 15% serum-containing medium (Serum), serum-free medium (SF) with or without 20nM myostatin (Mstn), for 2 h. Data are expressed as mean±standard error of the mean of six wells in each group. The Dunnett's test was used to analyze the differences between SF and Serum or Mstn groups. *, ** Significant with respect to SF group (* P < 0.05; ** P < 0.01).

Similar to the results observed in the presence of serum, myostatin significantly increased Smad2 phosphorylation and FOXO1 expression in chick myotubes cultured under serum-free conditions, and no significant change was observed in the phosphorylation of Smad3, Akt, and AMPK, and in mRNA levels of MuRF-1 (Fig. 2). Moreover, no significant change was observed in FOXO1 protein levels and its phosphorylation (Fig. 2A). However, no significant change was observed in atrogin-1 mRNA levels (Fig. 2A). These results suggest that Smad activation did not enhance serum-free-induced upregulation of atrogin-1 expression.

Myostatin mRNA levels were dramatically decreased by myostatin treatment under serum-free conditions (Fig. 2B). Similarly, although no significant difference was observed, mRNA levels of myostatin decreased to 58% in myostatin-treated cells under serum-supplemented conditions (Supplementary Figure 1). Therefore, the present results suggest that myostatin expression is negatively regulated via myostatin-induced Smad activation in chicken skeletal muscle.

Discussion

A previous in vitro study using C2C12 myotubes showed that myostatin increases mRNA levels of FOXO1 and atrogin-1, but not MuRF-1 (McFarlane ). Similarly, overexpression of activin receptor-like kinase 5(which is activated by the binding of myostatin to an activin type II receptor and then phosphorylates Smads) or Smad3 increases the activity of atrogin-1 but not MuRF-1 promotor, in murine skeletal muscle (Goodman ; Sartori ). Smad3 can bind directly to DNA at the 5′-AAGAC-3′-sequence known as Smad-binding element, whereas Smad2 cannot bind directly to DNA (Matsuzaki 2011). However, Sartori showed that RNAi-mediated knockdown of Smad3 alone or of both Smad2 and Smad3 induces a 10% and 22% increase in the cross-sectional area of murine muscle fiber, respectively. Smad2, therefore, also appears to be involved in the inhibition of muscle growth. In this study, using chick embryonic myotubes, similar results were observed, except Smad3 phosphorylation. These findings therefore suggest that the myostatin/Smad pathway plays a role in regulating the expression of proteolysis-related factors in chicken skeletal muscles, but the contributing isoform may be different from that in mammalian ones.

Previous studies using mammalian cells have investigated the long-term (12–48 h) effects of myostatin (McFarlane ; Deng ; Lokireddy ). McFarlane showed that myostatin-induced promotion of atrogin-1 expression is dependent on FOXO1. Additionally, Lokireddy found that active Smad signaling is required for myostatin to increase the protein levels of FOXO1 and atrogin-1. In contrast, the present study investigated the relatively short-term (2 h) effects of myostatin. Therefore, the difference in incubation time might be one of the reasons why no significant change was observed in the levels of Akt and FOXO1. Importantly, the present study showed that myostatin induced Smad2 phosphorylation and atrogin-1 expression without affecting the Akt/FOXO1 pathway. Smads are known to cooperate with other DNA binding proteins to elicit specific transcriptional response (Shi and Massagué, 2003). For example, Smad2/3 can bind members of the FOXO family of transcription factors to regulate gene expression (Gumucio and Mendias, 2013). Therefore, the present results might provide new hypotheses, suggesting that Smads are able to promote atrogin-1 transcription in cooperation with FOXO1 independently of Akt-mediated regulation, and that Smad cooperates with other unknown factors to regulate atrogin-1 expression.

Serum-free treatment increases mRNA and protein levels of atrogin-1 and MuRF-1 and decreases phosphorylation of Akt and FOXO in C2C12 and L6 myotubes (Kim ; Sandri ), indicating that the increase in atrogin-1 and MuRF-1 expression is controlled by the Akt/FOXO pathway. However, a previous study in C2C12 myotubes showed that an AMPK activator increased atrogin-1 and MuRF-1 mRNA levels without affecting Akt phosphorylation (Egawa ). In the present study, phosphorylation of AMPK, but not of FOXO1, was significantly induced by serum-free treatment with the increase in atrogin-1 and MuRF-1 expression. Therefore, it is possible that AMPK regulates atrogin-1 and MuRF-1 expression without affecting the Akt/FOXO pathway in both mammals and birds.

An AMPK activator reportedly increased the levels of myostatin protein in L6 myotubes (Lee ). Levels of myostatin mRNA significantly increased in skeletal muscles of Smad3-null mice and in C2C12 myotubes treated with a Smad3 inhibitor (McFarlane ). In the present study, AMPK appeared to increase myostatin expression in chick myotubes, whereas Smad appeared to inhibit myostatin expression even when AMPK was activated. Therefore, these findings suggest that AMPK and Smad control myostatin expression in chicken myotubes cultured in vitro, in the same manner as seen in mammals. In contrast to the results from in vitro studies, previous in vivo studies have suggested a different mechanism for myostatin expression in the skeletal muscle, between mammals and chickens. Fasting significantly promoted myostatin expression in mice (Allen ) and inhibited its expression in chickens (Guernec ; Saneyasu ). Although the exact reason for this difference remains unknown, based on the present results, fasting-induced decrease in myostatin expression in chicken skeletal muscle might be caused by the activation of the Smad signaling pathway. Interestingly, a previous study found that myostatin is present extracellularly in murine skeletal muscle as uncleaved pro-myostatin and proposed that extracellular cleavage of pro-myostatin to mature myostatin represents a novel control point for myostatin signaling in the skeletal muscle (Anderson ). With respect to TGF-β, activation of latent complexes is being increasingly recognized as a critical step in the control of TGF-β activity (Hayashi and Sakai, 2012). Indeed, in intact adult tissues and organs, TGF-β is secreted in a biologically inactive (latent) form associated in a non-covalent complex with the extracellular matrix, and the expression of TGF-β mRNA and protein levels do not often correlate with active TGF-β levels (Hayashi and Sakai, 2012). It is therefore possible that fasting affects the activation of latent myostatin in chicken skeletal muscle and then the increase in the active form inhibits its expression via upregulation of Smad phosphorylation.

The present study showed a discrepancy in atrogin-1 expression between the serum-supplemented and serum-free conditions. Although the exact reason is unclear, one possible explanation is that Smad-mediated upregulation of atrogin-1 might be limited under conditions of low AMPK activity in chick myotubes and as shown in the present study, this could be because myostatin induced Smad2 phosphorylation, but did not upregulate atrogin-1 expression under conditions of the high phosphorylation rate of AMPK, induced by serum-free treatment. Another possible explanation is that growth factors in the serum influence Smad-mediated gene transcription. Further studies are required to clarify the molecular mechanism underlying myostatin/Smad-induced transcription of atrogin-1.

In summary, significant increase was observed in Smad2 phosphorylation and atrogin-1 mRNA levels in myostatin-treated chick myotubes, whereas no significant change was observed in the phosphorylation of Akt and FOXO1, and MuRF-1 mRNA levels. These results suggest that myostatin upregulates atrogin-1 transcription by Smad activation in an Akt/FOXO pathway-independent manner in chicken skeletal muscles, which might be different from the mechanism observed in mammalian skeletal muscles.