The ketoacid analog ketosteril (KT; as compound α-ketoacid tablets) was purchased from Fresenius Kabi Asia-Pacific, Ltd. (Hong Kong SAR, China). APS, tumor necrosis factor (TNF)-α and the NF-κB inhibitor pyrrolidine dithiocarbamate (PDTC) were purchased from Sigma-Aldrich (Merck KGaA, Darmstadt, Germany). Other common laboratory reagents were purchased as reagent-grade from Sinopharm Chemical Reagent Co., Ltd. (Shanghai, China).

A total of 32 male Sprague-Dawley rats (7–8 weeks old, 250–300 g) were obtained from the Shanghai SLAC Laboratory Animal Co., Ltd. (Shanghai, China). The animal experiments in the current study were approved by the Shanghai Animal Care and Use Committee, Shanghai Institute of Materia Medica, Chinese Academy of Sciences [Certificate number, SCXK (Shanghai) 2002–0010; Shanghai, China]. Rats were housed at a temperature of 22±1°C and humidity of 55±5%. They were fed once a day and housed under a 12 h light/dark cycle with free access to water. Animals fasted for 12 h before sacrifice.

After a 3-day adaptation period, rats were divided into four groups (n=8 rats in each group). Three groups under-went 5/6 subtotal nephrectomy to establish a rat model of CRF-induced cachexia, as previously described (14). Of the three CRF rat groups, one group received treatment with APS (intraperitoneally, 3 g/kg/day) for 6 weeks and one group received treatment with KT (intravenously, 0.14 g/ml suspension, l ml/200 g/day) for 4 weeks. The third group received treatment with saline solution (intraperitoneally, 3 g/kg/day). Rats in the fourth group acted as a negative control without any renal damage but receiving saline solution (intraperitoneally, 3 g/kg/day). Following treatments for 6 weeks, femur skeletal muscle tissues from mice under sodium pentobarbital anesthesia (intraperitoneal, 40 mg/kg) were collected and stored at −80°C until use for further biochemistry analysis.

Rat L6 myoblasts were purchased from the American Type Culture Collection (Manassas, VA, USA) and maintained in high-glucose Dulbecco's modified Eagle's medium supplemented with 10% heat-inactivated fetal bovine serum and 1% antibiotic-antimycotic solution (cat. no. 15240096; Invitrogen; Thermo Fisher Scientific, Inc., Waltham, MA, USA) at 37°C in a humidified atmosphere of 95% air and 5% CO₂ for 24 h. An L6 muscle cell malnutrition model was induced by pretreatment with TNF-α (10 ng/ml) for 24 h at 37°C, as described previously (15).

After washing twice with PBS solution (0.01 M) twice for 2 min, 1.2×10⁶ L6 cells were treated with APS (15 mg/l) or PDTC (50 µmol/l) or PBS as a control for 48 h following induction of malnutrition at 37°C. Ten randomly selected fields were observed using an inverted microscope (Olympus Corporation, Tokyo, Japan) and the transaction diameter values of all four groups were measured prior to cell harvesting, as previously described (16).

L6 myoblasts treated with APS or PDTC, or PBS as a control, as described above, were seeded into 6-well plates in high-glucose Dulbecco's modified Eagle's medium supplemented with 10% heat-inactivated fetal bovine serum and 1% antibiotic-antimycotic solution (cat. no. 15240096; Invitrogen; Thermo Fisher Scientific, Inc.) at a density of 3×10⁵ cells/well and incubated for 1 day at 37°C. Cells in each well were then transfected with a full-length atrogin-1-siRNA (5′-CTACGTAGTAAGGCTGTTG-3′) transfection mix (100 µl Lipofectamine 2000 in a final volume of 1 ml cell medium; Shanghai GeneChem Co., Ltd., Shanghai, China) for 72 h at 37°C, according to the manufacturer's protocol, and incubated for 72 h at 37°C. All knockdown experiments were performed in triplicate.

Total RNA from tissues was isolated using a UNIQ-10 column and a TRIzol total RNA isolation kit (both from Sangon Biotech Co., Ltd., Shanghai, China) after fully grinding on ice for 10 min. Total RNA from cells was also isolated using a UNIQ-10 column and a Trizol total RNA isolation kit. Reverse transcription was performed using 1 µg total RNA in a reaction volume of 20 µl with cloned AMV reverse transcriptase (Invitrogen; Thermo Fisher Scientific, Inc.). A total of 2 µl cDNA was used for qPCR using a Takara Ex Taq RT-PCR Version 2.1 kit (Takara Bio, Inc., Otsu, Japan). The following gene-specific PCR primers (Sangon Biotech Co., Ltd.) were used: atrogin-1 were forward, 5′-AGCTTGTGCGATGTTACCA-3′ and reverse, 5′-GGTGAAAGTGAGACGGAGCA-3′; ubiquitin were forward, 5′-TCAGATGTGGAGAAAGGAGGG-3′ and reverse, 5′-GTTGAGCCGGCTGAGTTGAT-3′; β-actin were forward, 5′-CATTGCTGACAGGATGCAG-3′ and reverse, 5′-CTGCTGGAAGGTGGACAGTGA-3′. PCR signals were detected with a DNA Engine Opticon^® 2 Continuous Fluorescence Detection system (Bio-Rad Laboratories, Inc., Hercules, CA, USA). PCR conditions were as follows: An annealing temperature of 60°C, followed by 40 cycles of 94°C for 20 sec, 58°C for 20 sec and 72°C for 20 sec. Melt curve analysis and electrophoresis in 2% agar were performed in three replicates to evaluate the purity of PCR products. Negative control reactions (no template DNA) were included to monitor potential contamination of reagents. Relative amounts of atrogin-1 and ubiquitin mRNA were normalized to that of β-actin using the 2^−ΔΔCq method (17).

The concentrations of the protein extracts obtained from rat skeletal muscle tissue and L6 cells were determined using a bicinchoninic acid kit (Pierce; Thermo Fisher Scientific, Inc.) according to the manufacturer's protocols. Protein lysates (30 µg) were then separated on a 10% SDS-PAGE gel followed by transfer to nitrocellulose membranes (Bio-Rad Laboratories, Inc.). Western blot analysis was performed according to a standard protocol (18) using primary antibodies against atrogin-1 (cat. no. ab74023, 1:10,000; Abcam, Cambridge, UK), ubiquitin (cat. no. sc-4316, 1:1,000) and NF-κB subunit p65 (cat. no. c-20, 1:2,000; both from Santa Cruz Biotechnology, Inc., Dallas, TX, USA), and GAPDH (cat. no. A3853, 1:10,000; Sigma-Aldrich; Merck KGaA). Horseradish peroxidase conjugated mouse anti-rabbit IgG (sc-2357, 1:5,000; Santa Cruz Biotechnology, Inc.) was used as a secondary antibody. Resulting protein signals were detected using an enhanced chemiluminescence system (EMD Millipore, Billerica, MA, USA) and data was analyzed using the Stata 7.0 software package (StataCorp LLC, College Station, TX, USA). Three replicates were performed for each experiment.

Data are expressed as the mean ± standard deviation. Differences between groups were assessed using the Student's t-test and one-way analysis of variance followed by the Tukey's post hoc test in SPSS 19.0 (IBM SPSS, Armonk, NY, USA). Differences were considered to be statistically significant when P<0.05.

Western blot analysis indicated that expression of atrogin-1 and ubiquitin protein was markedly decreased in CRF rats treated with KT (intravenously, 0.14 g/ml suspension; l ml/200 g/day) or APS (intraperitoneally, 3 g/kg/day), compared with untreated CRF rats (Fig. 1A). Results from RT-qPCR indicated that levels of atrogin-1 (Fig. 1B) and ubiquitin (Fig. 1C) mRNA in CRF rats treated with KT were significantly decreased relative to untreated CRF rats (P<0.05). Treatment with APS also reversed the rise in astrogin-1 and ubiquitin protein expression (Fig. 1A), and significantly reversed the elevated levels of atrogin-1 and ubiquitin (both P<0.05; Fig. 1B and C) in CRF rats. In comparison to the normal control group, CRF rats treated with KT or APS, exhibited significantly increased expression of atrogin-1 and ubiquitin mRNA (P<0.05; Fig. 1B and C).

A state of cell malnutrition (cachexia) was established in vitro by pretreating rat L6 myoblasts with TNF-α (10 ng/ml). Atrogin-1-siRNA was also used to inhibit atrogin-1 expression. Efficiency of atrogin-1-siRNA transfection has been confirmed by western blot analysis and RT-qPCR (data not shown). Results indicated that the elevated levels of atrogin-1 and ubiquitin observed in TNF-α treated L6 myoblasts were reversed following administration of APS (Fig. 2A). NF-κB subunit p65 was also measured, and a lower level of protein expression was observed in L6 myoblasts following TNF-α + APS and TNF-α + atrogin-1-siRNA treatment compared with TNF-α treatment alone (Fig. 2A). Furthermore, RT-qPCR demonstrated that the elevated levels of atrogin-1 (Fig. 2B) and ubiquitin (Fig. 2C) mRNA induced by TNF-α were significantly reversed 48 h following administration of APS (P<0.05). In comparison to the normal control group, TNF-α + APS treated L6 myoblasts and TNF-α + atrogin-1-siRNA-treated L6 myoblasts exhibited significantly increased expression of atrogin-1 and ubiquitin mRNA (P<0.05; Fig. 2B and C).

It was observed by fluorescence microscopy that L6 myoblasts treated with TNF-α alone were atrophic, while cell sizes in the TNF-α + APS treatment group and TNF-α + atrogin-1-siRNA appeared unaffected, compared with normal control cells (Fig. 3A). In addition, relative to the TNF-α treatment group, the transverse diameters of the L6 myoblasts in the APS + TNF-α and atrogin-1-siRNA + TNF-α groups were significantly increased (P<0.05; Fig. 3B). TNF-α + APS treated L6 myoblasts and atrogin-1-siRNA + TNF-α treated L6 myoblasts had significantly decreased transverse diameters compared with the control group, ~70 and 90% of the control transverse diameter, respectively (both P<0.05; Fig. 3B).

At the protein level, it was observed that the elevated levels of atrogin-1, ubiquitin and p65 induced by TNF-α were markedly reduced by PDTC (Fig. 4A). Similarly, analysis of mRNA expression indicated that upregulation of atrogin-1 (Fig. 4B) and ubiquitin (Fig. 4C) mediated by TNF-α was significantly inhibited 48 h following administration of PDTC. In comparison with the normal control group, the TNF + PDTF group exhibited significantly increased expression of atrogin-1 and ubiquitin mRNA (both P<0.05).

Inverted fluorescent microscopy demonstrated that L6 rat myoblasts treated with TNF-α alone were atrophic compared with normal control cells, while cell sizes in the TNF-α + PDTC treatment group appeared unaffected (Fig. 5A). In addition, relative to the TNF-α treatment group, the transverse diameters of the L6 myoblasts in the PDTC + TNF-α group were significantly increased. In comparison with the normal control group, TNF+PDTF group had a significantly reduced transverse diameter (~90% relative to control group; P<0.05; Fig. 5B).