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MUSCLE CELL BIOLOGY AND CELL MOTILITY

TNF induction of atrogin-1/MAFbx mRNA depends on Foxo4 expression but not AKT-Foxo1/3 signaling

¹Department of Physiology, University of Kentucky, Lexington, Kentucky; and ²Department of Kinesiology, University of Toledo, Toledo, Ohio

Submitted 29 January 2008 ; accepted in final form 5 August 2008

	ABSTRACT

TOP ABSTRACT EXPERIMENTAL PROCEDURES RESULTS DISCUSSION GRANTS REFERENCES

 
Murine models of starvation-induced muscle atrophy demonstrate that reduced protein kinase B (AKT) function upregulates the atrophy-related gene atrogin-1/MAFbx (atrogin). The mechanism involves release of inhibition of Forkhead transcription factors, namely Foxo1 and Foxo3. Elevated atrogin mRNA also corresponds with elevated TNF in inflammatory catabolic states, including cancer and chronic heart failure. Exogenous tumor necrosis factor (TNF) increases atrogin mRNA in vivo and in vitro. We used TNF-treated C2C12 myotubes to test the hypothesis that AKT-Foxo1/3 signaling mediates TNF regulation of atrogin mRNA. Here we confirm that exposure to TNF increases atrogin mRNA (+125%). We also confirm that canonical AKT-mediated regulation of atrogin is active in C2C12 myotubes. Inhibition of phosphoinositol-3 kinase (PI3K)/AKT signaling with wortmannin reduces AKT phosphorylation (–87%) and increases atrogin mRNA (+340%). Activation with insulin-like growth factor (IGF) increases AKT phosphorylation (+126%) and reduces atrogin mRNA (–15%). Although AKT regulation is intact, our data suggest it does not mediate TNF effects on atrogin. TNF increases AKT phosphorylation (+50%) and stimulation of AKT with IGF does not prevent TNF induction of atrogin mRNA. Nor does TNF appear to signal through Foxo1/3 proteins. TNF has no effect on Foxo1/3 mRNA or Foxo1/3 nuclear localization. Instead, TNF increases nuclear Foxo4 protein (+55%). Small interfering RNA oligos targeted to two distinct regions of Foxo4 mRNA reduce the TNF-induced increase in atrogin mRNA (–34% and –32%). We conclude that TNF increases atrogin mRNA independent of AKT via Foxo4. These results suggest a mechanism by which inflammatory catabolic states may persist in the presence of adequate growth factors and nutrition.

skeletal muscle; cachexia; atrophy; ubiquitin; cytokines

Atrogin gene expression is under the transcriptional control of Forkhead box O transcription factors (Foxo). Foxo1, Foxo3, and Foxo4 are related Foxo proteins thought to regulate atrogin under a variety of conditions. Foxo1 and Foxo3 mRNA are upregulated with starvation (21, 24), diabetes (26), cachexia, and aging (13, 22, 24). Foxo4 is less well studied but is modulated in heart failure models of atrophy (42).

Foxo1, Foxo3, and Foxo4 activity is regulated by phosphoinositol-3 kinase (PI3K)-protein kinase B (AKT) signaling (41, 42, 45). Basal AKT function maintains Foxo in a phosphorylated state that favors cytoplasmic retention and repression of transcriptional activity. Overexpression of IGF can further suppress Foxo activity through stimulation of AKT (15, 16, 42). Wortmannin, a PI3K inhibitor, depresses AKT activity and Foxo phosphorylation (28, 40, 44). With starvation or dexamethasone treatment, AKT activity and Foxo1 and Foxo3 phosphorylation are decreased. Foxo1/3 subsequently translocate to the nucleus to drive atrogin expression (41, 45). The activity of Foxo4 under these conditions has not been established.

Atrogin mRNA has been shown to increase with tumor necrosis factor (TNF) exposure in muscles of rats (12) and mice (31) and in primary and C2C12 myotubes (30, 31). The goal of our current study was to define components of the signaling pathway that mediate TNF-induced atrogin expression. We postulated that a similar AKT-Foxo1/3-dependent mechanism mediates TNF effects on atrogin expression in differentiated muscle cells. This model (Fig. 1A) was evaluated by using mature C2C12 myotubes to test two hypotheses: 1) TNF induces atrogin expression through inhibition of AKT. To assess the role of AKT, we measured changes in atrogin expression and AKT phosphorylation after a time course of TNF exposure. We also measured the inhibitory potential of AKT activation on TNF-induced atrogin expression. 2) TNF induces atrogin expression through activation of Foxo1/3 transcription factors. To assess the roles of Foxo1, Foxo3, and Foxo4, we measured changes in Foxo mRNA, protein, and nuclear translocation after TNF exposure.

View larger version (20K): [in this window] [in a new window]   Fig. 1. Model of regulation of atrogin by tumor necrosis factor- (TNF). A: inhibition of protein kinase B (AKT) leads to activation of Forkhead box O transcription factor (Foxo) and an increase in atrogin mRNA. We hypothesized that TNF might increase atrogin expression by inhibiting AKT. B: we propose TNF increases atrogin expression by overriding the inhibitory effects of AKT and activating Foxo4 by an unknown mechanism. atrogin, atrogin-1/MAFbx muscle atrophy F-box; IGF, insulin-like growth factor; PI3K, phosphoinositide 3-kinase.

	EXPERIMENTAL PROCEDURES

TOP ABSTRACT EXPERIMENTAL PROCEDURES RESULTS DISCUSSION GRANTS REFERENCES

 
Cell culture. C2C12 myoblasts (American Type Culture Collection, Rockville, MD) were seeded at a density of 8,000–10,000 cells/cm² and allowed to proliferate in Dulbecco's modified Eagle's medium supplemented with 10% fetal bovine serum and 25 mg/ml gentamicin (GIBCO-Invitrogen, Carlsbad, CA) in 5% CO₂ at 37°C. After 2 days the myoblasts were shifted to differentiation medium (Dulbecco's modified Eagle's medium-2% horse serum-25 mg/ml gentamicin). After 4–6 days of differentiation, myotubes were treated with the following reagents: 6 ng/ml recombinant mouse TNF (Pierce, Rockford, IL), 10 ng/ml recombinant human IGF-1 (Invitrogen), 100 nM wortmannin (Sigma-Aldrich, St. Louis, MO), or 1 µM 4-hydroxytamoxifen (Sigma-Aldrich).

Stable Foxo1/TSS-ER C2C12 cell lines were generated according to Bastie et al. (1). Briefly, the AKT phosphorylation sites in Foxo1 (Thr24, Ser256, and Ser319) were mutated to alanine. The COOH-terminus was fused to a modified ligand-binding domain of the estrogen receptor. This ligand-binding domain is transcriptionally inactive and has been mutated such that it specifically responds to tamoxifen but not to endogenous estrogens (33). The construct was cloned into the pBABE retroviral vector containing the puromycin selection marker and stably transfected cells were isolated.

Relative quantification real time PCR (rqPCR). Reverse transcription was performed with Murine-Maloney leukemia virus reverse transcriptase and random hexamers (Promega, Madison, WI) plus 2 µg total RNA isolated with TRIzol reagent (Invitrogen). The mouse cDNA sequences for atrogin-1/MAFbx (NM-026346), Foxo1 (NM-019739.2), Foxo3 (NM-019740.2), Foxo4 (Mllt7, NM-018789.1), and β-actin (NM-007393.1) were obtained from GenBank. PCR primers were designed from the cDNA sequences using Primer Express 1.5 software (Applied Biosystems, Foster City, CA). Primer sequences are as follows: atrogin forward 5'-ATGCACACTGGTGCAGAGAG-3'; reverse; 5'-TGTAAGCACACAGGCAGGTC-3' Foxo1 forward 5'-GTGAACACCAATGCCTCACAC-3', reverse 5'-CACAGTCCAAGCGCTCAATA-3'; Foxo3 forward 5'-AGCCGTGTACTGTGGAGCTT-3', reverse 5'- TCTTGGCGGTATATGGGAAG-3'; Foxo4 forward 5'-CAAGAAGAAGCCGTCTGTCC-3', reverse 5'-CTGACGGTGCTAGCATTTGA-3'; b-actin forward 5'-AGGCCCAGAGCAAGAGAGGTA-3', reverse 5'-CCATGTCGTCCCAGTTGGTAA-3'. Synthesized primers were purchased from Invitrogen. PCR was performed using Applied Biosystems 7500 Real Time PCR system. Targets were amplified from 50 ng of cDNA using SYBR Green Master Mix reagent (stage 1, 1 cycle, 50°C, 2 min; stage 2, 1 cycle, 95°C, 10 min; stage 3, 40 cycles, 95°C, 15 s, 60°C, 1 min; Applied Biosystems). Reactions were performed in duplicate or triplicate for each cDNA sample. The abundance of target mRNA relative to β-actin mRNA was determined using the comparative cycle threshold method (14, 34).

Western blot analysis. Cells were washed once with phosphate-buffered saline (PBS) then resuspended and briefly sonicated in 2x sample loading buffer (120 mM Tris, pH 7.5, 200 mM DTT, 20% glycerol, 4% SDS, and 0.002% bromphenol blue). Proteins were fractionated on 4–15% SDS-polyacrylaminde gels (Criterion precast gels, Bio-Rad, Hercules, CA). Fractionated proteins were transferred to reduced-fluorescence polyvinyldifluoride membrane (Immobilon-FL, Millipore, Bedford, MA). Membranes with transferred proteins were blocked for 1 h at room temperature in Odyssey Blocking Buffer (LI-COR, Lincoln, NE). Primary antibodies were incubated overnight at room temperature in Odyssey Blocking Buffer mixed 1:1 with PBS plus 0.2% Tween. Secondary antibodies were incubated for 30 min in Odyssey-PBS-0.2% Tween plus 0.01% SDS. Total AKT antibody and atrogin antibody were purchased from ECM Biosciences (Versailles, KY). Foxo1, Foxo4, and phospho-specific AKT (S473) antibodies were purchased from Cell Signaling Technologies (Danvers, MA). Foxo3 antibody was purchased from Upstate (Lake Placid, NY). Myosin antibody was from Sigma. Fluorescent secondary antibodies were used for detection (goat anti-mouse Alexa-680, Molecular Probes-Invitrogen; goat anti-rabbit IRD800, Rockland Immunochemicals, Gilbertsville, PA). Fluorescence was imaged and results were quantified using the Odyssey Infrared Imaging System (LI-COR).

Immunocytochemistry. Foxo1/TSS overexpressing C2C12 skeletal myotubes were grown on glass coverslips coated in ECL cell attachment matrix (Upstate, Charlottesville, VA) for 4 days in DMEM supplemented with 2% horse serum (Invitrogen). Foxo1/TSS myotubes were treated with either vehicle (0.1% vol/vol EtOH final concentration) or 1 µM 4-hydroxytamoxifen (4-HT) for 2 h. Myotubes were then washed in PBS, fixed in 4% formaldehyde in PBS, permeabilized (0.5% Triton X-100 in PBS), blocked (1 M Tris·HCl, pH 7.6, supplemented with 3% BSA, 0.2% gelatin, 0.05% Tween-20), and incubated overnight at 4°C with primary antibody directed against the Foxo1 protein (Cell Signaling). Myotubes were then washed in PBS, incubated with a TRITC-conjugated secondary antibody (Jackson Immuno Research, West Grove, PA), and mounted in Vectashield mounting medium supplemented with 4',6-diamidino-2-phenylindole (Vector Labs, Burlingame, CA). Myotubes were assessed for Foxo1 localization using a Zeiss LSM 510 confocal microscope (Carl Zeiss MicroImaging, Thornwood, NY).

siRNA. Two Silencer predesigned siRNAs for Foxo4 (siRNA IDs: no. 184930 and no. 184932) and Negative Control no. 2 siRNA were purchased from Ambion (Austin, TX). siRNA (100 µM) was transfected into day 4 myotubes using oligofectamine diluted 1:5 with DMEM according to the manufacturer's instructions (Invitrogen). Changes in atrogin mRNA and protein were assayed 72 h posttransfection.

Statistical analysis. Data were normally distributed and are expressed as means ± SE. Student's t-test was used for the statistical comparison of two means; ANOVA was used for the comparison of multiple means. When ANOVA revealed significant differences, Tukey's post hoc test for multiple comparisons was performed. *P values <0.05 were considered significant.

	RESULTS

TOP ABSTRACT EXPERIMENTAL PROCEDURES RESULTS DISCUSSION GRANTS REFERENCES

 
TNF modulation of atrogin. TNF regulation of atrogin mRNA and the effect on myosin levels was measured by real time PCR and Western blot analysis. Atrogin mRNA increases early and peaks at 2 h. A decrease in myosin protein is detected after 72 h of daily TNF treatments (Fig. 2A). These data confirm earlier reports that show TNF induces atrogin expression (30) and myosin loss (8, 32). In addition, our data are the first to show that TNF causes an elevation in atrogin protein that begins to accumulate by 6 h (Fig. 2A) and remains elevated with chronic, repeated exposure to TNF (Fig. 2B).

View larger version (19K): [in this window] [in a new window]   Fig. 2. TNF regulation of atrogin. A: C2C12 myotubes were treated with 6 ng/ml TNF for 1, 2, 4, and 6 h. Atrogin mRNA was measured by real-time PCR, and protein was measured by Western blot analysis (insets). mRNA increased by 1 h and peaked at 2 h, protein peaked by 6 h (*P < 0.05 vs. untreated control, n = 3). B: C2C12 myotubes were treated chronically with 6 ng/ml TNF added at 24, 48, and 72 h. Atrogin protein remained elevated and myosin levels dropped (*P < 0.05 vs. untreated control, n = 3).

View larger version (22K): [in this window] [in a new window]   Fig. 3. Canonical AKT pathway regulation of atrogin. C2C12 myotubes were treated with wortmannin 100 nm (A), IGF 10 ng/ml (B) for 2 h, or subjected to overexpression of a Foxo1/TSS mutant resistant to inhibition by AKT (C). This mutant is fused to the ligand-binding domain of the estrogen receptor and was induced to translocate to the nucleus with 4-hydroxytamoxifen (4-HT, 1 µM). AKT was measured by immunoblotting with antibodies specific for total and phospho-AKT. AKT phosphorylation decreased with wortmannin and increased with IGF (*P < 0.001, n = 3). Atrogin mRNA was measured by real time PCR. Atrogin increased with wortmannin and 4-HT induced Foxo1/TSS nuclear translocation (*P < 0.001, n = 3) and decreased with IGF (*P < 0.05, n = 3). 4-HT had no effect on atrogin mRNA in vector control cells.

View larger version (26K): [in this window] [in a new window]   Fig. 4. TNF-induced atrogin expression and AKT activation. A: C2C12 myotubes were treated with 6 ng/ml TNF for 15 and 30 min and 2 and 6 h. AKT was measured by immunoblotting with antibodies specific for total and phospho-AKT. AKT phosphorylation is evident by 15 min and persists for up to 2 h (*P < 0.05, n = 3). B: myotubes were pretreated for 30 min with 10 ng/ml IGF followed by 2 h TNF 6 ng/ml. As measured by Western blot analysis and real time PCR, pretreatment with IGF elevates phospho-AKT levels eightfold relative to TNF alone (**P < 0.0001, n = 3) but does not prevent the TNF-induced rise atrogin mRNA.

View larger version (19K): [in this window] [in a new window]   Fig. 5. Basal Foxo isoform levels and localization. A: total RNA from untreated C2C12 myotubes was extracted and assayed by real time PCR for Foxo1, Foxo3, and Foxo4 mRNA. B: nuclear (nuc) and cytoplasmic (cyt) extracts were prepared from untreated C2C12 myotubes, and Foxo localization was measured by Western blot analysis with antibodies specific for Foxo1, Foxo3, and Foxo4. Basal Foxo1 and Foxo3 protein are approximately evenly distributed between cytoplasmic and nuclear compartments. Foxo4 is predominantly cytoplasmic (P < 0.01 nuclear vs. cytoplasmic Foxo4, n = 3).

View larger version (17K): [in this window] [in a new window]   Fig. 6. Foxo isoform response to TNF. A: C2C12 myotubes were treated with 6 ng/ml TNF for 2 h; total RNA was isolated and assayed by real time PCR for changes in Foxo1, Foxo3, and Foxo4 mRNA. Foxo isoform mRNAs did not change with TNF. B: nuclear and cytoplasmic extracts were prepared from TNF-treated C2C12 myotubes, and Foxo isoform localization was measured by Western blot analysis with antibodies specific for Foxo1, Foxo3, and Foxo4. Only Foxo4 translocates to the nucleus in response to TNF (*P < 0.05).

View larger version (25K): [in this window] [in a new window]   Fig. 7. Downregulation of Foxo4 diminishes the induction of atrogin mRNA in response to TNF. Small interfering RNAs (siRNAs) 100 µM specific to 2 regions of the Foxo4 mRNA and a nonspecific siRNA control (siFoxo4-0, siFoxo4-2, and NS) were transfected into myotubes 96 h postdifferentiation. Seventy-two hours posttransfection, myotubes were treated for 2 h with 6 ng/ml TNF. A: Foxo4 mRNA, as assayed by real time PCR, and protein, as assayed by Western blot analysis, were reduced by both siFoxo4-0 and siFoxo4-2 relative to the nonspecific siRNA control (*P < 0.05, n = 3). B: TNF-induced increase in atrogin mRNA, as measured by real time PCR, was reduced by siFoxo4-0 and siFoxo4-2 relative to the nonspecific siRNA control (34% average reduction, *P < 0.05, n = 3). C: linear regression showing the relationship between changes in Foxo4 protein and changes in atrogin mRNA.

View larger version (32K): [in this window] [in a new window]   Fig. 8. IGF effects on Foxo4. Myotubes were pretreated for 30 min with 10 ng/ml IGF followed by 2 h 6 ng/ml TNF. A: as measured by Western blot, pretreatment with IGF elevates phospho-Foxo4 (*P < 0.01, n = 3), and TNF does not reverse IGF-induced phosphorylation. B: nuclear extracts were prepared from myotubes treated as in A. TNF induced Foxo4 nuclear translocation (*P < 0.05, n = 3) that was not prevented by pretreatment with IGF.

	DISCUSSION

TOP ABSTRACT EXPERIMENTAL PROCEDURES RESULTS DISCUSSION GRANTS REFERENCES

Our results suggest that neither Foxo1 nor Foxo3 respond to TNF. Instead, Foxo4 appears to be the TNF-responsive isoform. Under basal conditions Foxo4 protein is mostly restricted to the cytoplasm and TNF rapidly stimulates nuclear translocation. Knockdown of Foxo4 protein by siRNA represses TNF regulation of atrogin. These data prompted us to refine our model and propose that Foxo4 mediates TNF-induced atrogin expression. Our results are reinforced by data from mouse models of heart failure, a pathophysiological process accompanied by chronic inflammation. Twelve weeks after induction of heart failure, animals exhibit skeletal muscle atrophy with increased active Foxo4 protein and elevated atrogin mRNA (42). Further experiments with Foxo4-null mice or cells stably transfected with Foxo4 shRNA will be important to better define the role Foxo4 plays in atrophy associated with chronic inflammation.

There are several potential mechanisms by which TNF might activate Foxo4. Among these, response to changes in intracellular oxidant activity is a common regulatory theme. Skeletal muscle oxidant activity is elevated in chronic inflammatory states or with exposure to TNF (18, 36). These increases in cellular oxidant activity are thought to be pro-catabolic (38, 36) and can activate Foxo4 by at least four mechanisms. First, Foxo factors are subject to regulation by redox-sensitive reversible acetylation (23). Acetylation, which inhibits Foxo transcriptional activity, is catalyzed by histone acetyltransferase cAMP-response element-binding protein-binding protein (5). Oxidative stress releases this inhibition by deacetylation via NAD-dependent deacetylase hSir2 (SIRT1) (23, 48). Second, oxidative stress can stimulate rapid monoubiquitination of Foxo4, causing nuclear translocation and increased transcriptional activity in human embryonic kidney cells (47). Third, H₂O₂ or TNF treatment of fibroblasts increases activation of Foxo4 via jun NH₂-terminal kinase (JNK)-dependent phosphorylation of threonines 447 and 451 (11). JNK is also activated by H₂O₂ or TNF in cultured myotubes (30), suggesting JNK could mediate TNF/Foxo4 signaling in muscle. Finally, Li et al. (30) demonstrated that TNF-induced atrogin expression is dependent on p38 mitogen-activated protein kinase (p38 MAPK). Like JNK, p38 MAPK activity is increased by H₂O₂ or TNF in skeletal muscle myotubes, and suppression of this activity prevents the induction of atrogin (30).

The signaling mechanisms that regulate atrogin expression appear to differ depending on catabolic stimulus. AKT regulation of atrogin is modulated by low nutrients, dexamethasone, or pharmacological inhibition. All of these reduce AKT activity, relieving Foxo1, Foxo3 (41, 45), and presumably Foxo4 inhibition. TNF and/or potentially inflammation in general appear to act via a second pathway. Our current findings indicate TNF increases Foxo4 activity through an AKT-independent, growth factor-insensitive process. Thus the TNF/Foxo4 pathway is a mechanism by which inflammation might upregulate atrogin and promote muscle catabolism despite high levels of circulating nutrients or growth factors. The intermediate steps in this pathway and the mechanism by which TNF bypasses AKT regulation of Foxo4 are yet to be defined.

	GRANTS

TOP ABSTRACT EXPERIMENTAL PROCEDURES RESULTS DISCUSSION GRANTS REFERENCES

 
This study was supported by National Heart, Lung, and Blood Institute Grant HL-59878.

	FOOTNOTES

 

Address for reprint requests and other correspondence: J. S. Moylan, Dept. of Physiology, Univ. of Kentucky, Lexington, KY 40536-0298 (e-mail: jennifer.moylan{at}uky.edu)

The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

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