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Leptin and leucine synergistically regulate protein metabolism in C2C12 myotubes and mouse skeletal muscles

Published online by Cambridge University Press:  05 December 2012

Xiangbing Mao
Affiliation:
State Key Laboratory on Animal Nutrition, China Agricultural University, No. 2, Yuanmingyuan West Road, Beijing100193, People's Republic of China
Xiangfang Zeng
Affiliation:
State Key Laboratory on Animal Nutrition, China Agricultural University, No. 2, Yuanmingyuan West Road, Beijing100193, People's Republic of China
Zhimin Huang
Affiliation:
State Key Laboratory on Animal Nutrition, China Agricultural University, No. 2, Yuanmingyuan West Road, Beijing100193, People's Republic of China
Junjun Wang
Affiliation:
State Key Laboratory on Animal Nutrition, China Agricultural University, No. 2, Yuanmingyuan West Road, Beijing100193, People's Republic of China
Shiyan Qiao*
Affiliation:
State Key Laboratory on Animal Nutrition, China Agricultural University, No. 2, Yuanmingyuan West Road, Beijing100193, People's Republic of China
*
*Corresponding author: S. Qiao, fax +86 10 6273 3688, email [email protected]
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Abstract

Leucine and leptin play important roles in regulating protein synthesis and degradation in skeletal muscles in vitro and in vivo. However, the objective of the present study was to determine whether leptin and leucine function synergistically in regulating protein metabolism of skeletal muscles. In the in vitro experiment, C2C12 myotubes were cultured for 2 h in the presence of 5 mm-leucine and/or 50 ng/ml of leptin. In the in vivo experiment, C57BL/6 and ob/ob mice were randomly assigned to be fed a non-purified diet supplemented with 3 % l-leucine or 2·04 % l-alanine (isonitrogenous control) for 14 d. Ob/ob mice were injected intraperitoneally with sterile PBS or recombinant mouse leptin (0·1 μg/g body weight) for 14 d. In C57BL/6 mice, dietary leucine supplementation increased (P< 0·05) plasma leptin, leptin receptor expression and protein synthesis in skeletal muscles, but reduced (P< 0·05) plasma urea and protein degradation in skeletal muscles. Dietary leucine supplementation and leptin injection increased the relative weight of the gastrocnemius and soleus muscles in ob/ob mice. Moreover, leucine and leptin treatments stimulated (P< 0·05) protein synthesis and inhibited (P< 0·05) protein degradation in C2C12 myotubes and skeletal muscles of ob/ob mice. There were interactions (P< 0·05) between the leucine and leptin treatments with regard to protein metabolism in C2C12 myotubes and soleus muscles of ob/ob mice but not in the gastrocnemius muscles of ob/ob mice. Collectively, these results suggest that leptin and leucine synergistically regulate protein metabolism in skeletal muscles both in vitro and in vivo.

Type
Full Papers
Copyright
Copyright © The Authors 2012 

As a functional amino acid, leucine can regulate protein metabolism in multiple tissues and cells, including skeletal muscles and myogenic cells, through insulin-dependent and -independent ways(Reference Anthony, Reiter and Anthony1Reference Li, Yin and Tan10). In addition, leucine treatment increases the expression of specific proteins in some tissues and cells including leptin in adipocytes and adipose tissues(Reference Lynch, Hutson and Patson11, Reference Roh, Han and Tzatsos12).

Leptin, a product of the obesity (ob) gene, is a 16 kDa hormone(Reference Zhang, Proenca and Maffei13), and is primarily expressed in the adipose tissue of multiple mammalian species(Reference Maffei, Halaas and Ravussin14). Leptin regulates many important physiological functions, including fatty acid metabolism, body temperature, reproduction, energy consumption, protein metabolism and insulin function(Reference Tartaglia15Reference Lamosová and Zeman19). However, leptin exerts its action via leptin receptors that are a type of transmembrane receptor.

Leptin receptors are the product of the diabetes (db) gene(Reference Tartaglia, Dembski and Weng20). There are at least six isoforms of leptin receptors produced by alternative splicing of the RNA transcript of the db gene(Reference Chua, Chung and Wu-Peng21). Leptin receptors are found in many mammalian tissues. Recent studies have shown that the expression of leptin receptors in specific tissues is affected by various nutrients and hormones(Reference Chen, Li and Yin22Reference Alonso, Fernández and Moreno24). We have recently shown that leucine promotes leptin receptor expression in C2C12 myotubes(Reference Mao, Zeng and Wang25). However, it has not been determined whether leucine can stimulate the expression of leptin receptors in vivo.

Several recent studies have alluded to potentially synergistic effects of different factors on some physiological functions(Reference O'Connor, Bush and Suryawan4, Reference Miyanaga, Ogawa and Ebihara26Reference Sadagurski, Norquay and Farhang30). Leucine or leptin has been shown to regulate protein metabolism in skeletal muscles. However, it is also possible that leucine and leptin can cross-talk in regulating protein metabolism in skeletal muscles. Therefore, the present study was conducted to test the hypothesis that leptin and leucine could synergistically regulate protein metabolism in mouse skeletal muscles and myogenic cells.

Materials and methods

Cell culture

C2C12 myoblasts (American Type Culture Collection) were used as an in vitro model for skeletal muscle and were cultured and differentiated into C2C12 myotubes as described previously(Reference Mao, Zeng and Wang25). Before the beginning of the treatment, the myotubes were starved for 12 h in serum- and antibiotic-free Dulbecco's modified Eagle's medium/F12, and the in vitro experiment was carried out in this starvation medium.

Measurement of protein synthesis and degradation in vitro

After starvation, the myotubes were cultured for 2 h in the presence of 5 mm-leucine and/or 50 ng/ml of leptin, and subsequently 2 μmol l-[2H5]phenylalanine (Cambridge Isotopes Laboratories) was added to each well without changing the medium. The supplemental levels of 5 mm-leucine and 50 ng/ml of leptin were chosen because they have been shown in previous studies and our preliminary study to regulate the protein metabolism of C2C12 myoblasts or myotubes(Reference Du, Shen and Zhu3, Reference Ramsay18, Reference Mao, Zeng and Wang25, Reference Berti and Gammeltoft31). Following incubation, the isotopic enrichment of l-[2H5]phenylalanine in the free pool and protein-bound pool of the myotubes was measured according to previously published procedures(Reference Wang, Qiao and Yin32, Reference Le Bacquer, Nazih and Blottière33). Ions with mass:charge ratios of 148 and 153 were monitored and converted to a percentage of molar enrichment (mol%) using calibration curves.

Protein degradation in the myotubes was determined by the release of tyrosine as described previously(Reference Nakashima, Ishida and Yamazaki8, Reference Ramsay18, Reference Kanazawa, Taneike and Akaishi34). Briefly, following starvation, the myotubes in six-well plates were incubated with 5 mm-leucine and/or 50 ng/ml of leptin for 2 h in the starvation medium. Then, the medium was immediately aspirated, and each well was washed two times with ice-cold sterile PBS. The C2C12 myotubes were incubated at 37°C for 6 h in a Krebs–Henseleit–HEPES buffer supplemented with 0·5 mm-pyruvate, 14·5 mm-glucose and 20 μm-cycloheximide. After incubation, the buffer was collected, and tyrosine concentration was analysed using an S-433D Amino Acid Analyser (Sykam), as described previously(Reference Zeng, Wang and Fan35). The myotubes were washed three times with ice-cold sterile PBS, and were dissolved in 1 m-NaOH. Proteins of the myotubes were assayed by the Lowry method using bovine serum albumin as the standard(Reference Lowry, Rosebrough and Farr36).

Mice and diets

All mice used in the present study were humanely managed according to the established guidelines of the China Department of Agriculture. The experimental protocol was approved by the China Agricultural University Animal Care and Use Committee (Beijing, China). C57BL/6 male mice weighing 13–15 g and leptin-deficient ob/ob male mice weighing 30–42 g were obtained from the Model Animal Research Center of Nanjing University (Nanjing, China). Mice were individually housed in a temperature- and light-controlled room with the temperature set at 21–23°C and the lighting schedule set at 12 h light–12 h dark. Food and water were available ad libitum.

A non-purified rodent diet based on maize, soyabean meal, wheat flour and fishmeal was obtained from Science Australia United Efforts Incorporation (Beijing, China; catalogue no. 2005-0007-Ka112). Either 3 % (w/w) l-leucine or 2·04 % (w/w) l-alanine (isonitrogenous control) was added to this non-purified rodent diet. Feed mixing was conducted by Science Australia United Efforts Incorporation (Beijing, China). The supplemental level of 3 % l-leucine was chosen because it has been shown in previous studies to regulate the protein metabolism of skeletal muscles, but not to affect the feed intake of mice or piglets(Reference Matsuzaki, Kato and Sakai37Reference Mao, Zeng and Cai39). Nutrient levels of the non-purified rodent diet were digestible energy (13·41 MJ/kg), protein (21·5 %, w/w), Ca (1·46 %, w/w), total P (0·92 %, w/w) and available P (0·75 %, w/w). The analysed contents (%, w/w) of amino acids in the leucine- and alanine-supplemented diets are summarised in Table 1.

Table 1 Analysed contents of amino acids (g/100 g) in the alanine- and leucine-supplemented non-purified rodent diets

+Ala, l-alanine-supplemented diet; +Leu, l-leucine-supplemented diet.

In vivo experimental design

After 3 d of acclimatisation, twenty C57BL/6 mice or twenty-four ob/ob mice were assigned on the basis of body weight to be fed the leucine-supplemented diet or the alanine-supplemented (isonitrogenous control) diet (n 10 or n 12). For 14 d, half of the ob/ob mice (n 6) on each diet were intraperitoneally injected with sterile PBS, while the other half were intraperitoneally injected with 0·1 μg/g body weight of a solution of recombinant mouse leptin dissolved in PBS. The injection dose of 0·1 μg/g body weight of leptin was chosen for 14 d because it was shown in previous studies to regulate physiological functions in ob/ob mice, but not to significantly affect their feed intake in the longer term(Reference Picard, Richard and Huang40, Reference Pelleymounter, Cullen and Baker41). The feed was supplied for every 7 d. In each supplying feed, the remaining feed and the supplied feed would be weighed, which was used to measure the feed intake of mice. On the morning of days 0 and 14, the body weight of mice was measured following a 12 h fast. On day 14, 1·5 h after feeding, mice received an intraperitoneal injection of a flooding dose of l-[2H5]phenylalanine (150 μmol/100 g body weight) as described previously(Reference Anthony, Reiter and Anthony1, Reference Schaefer and Scott42). At 30 min after the isotope administration, mice were anaesthetised with sodium pentobarbital, and blood samples were taken from the orbital sinus using vacutainer tubes coated with sodium heparin (Greiner Vacuette). Plasma was separated from the whole blood by centrifugation at 3000 g for 10 min, and stored at − 20°C until analysis. The left gastrocnemius and soleus muscles were excised, quickly frozen in liquid N2 and used for the determination of protein synthesis; Western blot and RNA isolate analyses were conducted as described later. The contralateral hindlimb muscles were also excised, weighed and used for the measurement of protein degradation.

Measurements of protein synthesis and degradation in muscles

Protein synthesis in muscle samples and the isotopic enrichment of l-[2H5]phenylalanine in the free and protein-bound pools were measured as described previously(Reference Wang, Qiao and Yin32, Reference Bregendahl, Liu and Cant43). Ions with mass:charge ratios of 148 and 153 were monitored and converted to the percentage of molar enrichment (mol%) using calibration curves.

Protein degradation of the gastrocnemius and soleus muscles was determined by the release of tyrosine as described previously(Reference Combaret, Dardevet and Rieu6, Reference Tawa and Goldberg44). Briefly, the intact gastrocnemius and soleus muscles were preincubated at 37°C in Krebs–Henseleit bicarbonate buffer supplemented with 5 mm-HEPES, 5 mm-glucose and 0·1 % bovine serum albumin, which was equilibrated with 95 % O2 and 5 % CO2, following the isolation of the muscles. After 30 min of preincubation, the muscles were transferred into fresh Krebs–Henseleit bicarbonate buffer containing 0·5 mm-cycloheximide, and further incubated at 37°C. The rate of protein degradation was determined by the release of tyrosine into the buffer containing cycloheximide in a 2 h period. Tyrosine was assayed using an S-433D Amino Acid Analyser (Sykam, GmbH), as described previously(Reference Zeng, Wang and Fan35).

Calculations

The fractional protein synthesis rate (FSR) in myotubes and skeletal muscles was calculated as: FSR (%/d) = (E Bound× 1440 × 100 %)/(E Free× t), where E Bound is the isotopic enrichment (%) of the tracer phenylalanine in the protein-bound pool at time t; 1440 is the number of min/d; E Free is the enrichment of the tracer phenylalanine in the free pool at time t; t is the exact time (min) of incubation with labelled phenylalanine(Reference Wang, Qiao and Yin32, Reference Le Bacquer, Nazih and Blottière33).

Plasma urea, amino acid and leptin measurement

Plasma urea was measured using an assay kit from Nanjing Jiancheng Biochemistry Institute. Plasma free amino acids were analysed using an S-433D Amino Acid Analyser (Sykam, GmbH) as described previously(Reference Zeng, Wang and Fan35). Leptin levels in plasma were determined using a mouse leptin ELISA kit (R & D Systems, Inc.).

Western blot analysis

Protein levels for β-actin and leptin receptor in skeletal muscles were determined by Western blot analysis as described previously(Reference Mao, Zeng and Wang25, Reference Suryawan, Nguyen and Bush45).

RNA isolation and quantitative real-time PCR

Total RNA was extracted from the skeletal muscles with the RNeasy Plus Mini Kit (Qiagen GmbH) according to the manufacturer's protocol. Then, RT of total RNA and quantitative real-time PCR of the β-actin and leptin receptor genes were conducted as described previously(Reference Mao, Zeng and Wang25).

Statistical analysis

Data for the C57BL/6 mouse experiment were analysed using the unpaired t test. Data for the C2C12 myotubes and ob/ob mouse experiments were analysed as a 2 × 2 factorial using the general linear model procedures of the Statistical Analysis System (SAS Institute). The factors in the models included the main effects of leucine treatment (supplemented or unsupplemented with leucine in the media or the diet) and leptin treatment (leptin or PBS supplementation) as well as their interaction. All analyses were performed using SAS (version 8.1; SAS Institute). Data are expressed as means with their standard errors, or means with their pooled standard errors. P< 0·05 was considered to indicate statistical significance.

Results

Effect of dietary leucine supplementation on growth performance and plasma concentrations of leptin, urea and amino acids in C57BL/6 mice

The feed intake, body-weight gain and feed conversion of C57BL/6 mice did not differ between mice fed the alanine- and leucine-supplemented diets (Table 2). However, leucine supplementation increased (P< 0·05) the plasma leptin concentration of C57BL/6 mice by 20 % (Fig. 1). Plasma urea concentration was 28 % lower in mice fed the leucine-supplemented diet compared with the alanine-supplemented diet (P< 0·05; Table 3). Moreover, leucine supplementation significantly increased plasma leucine concentration but decreased plasma concentrations of glutamate (P< 0·01), serine (P< 0·01), threonine (P< 0·01), tyrosine (P< 0·05) and valine (P< 0·01) in C57BL/6 mice (Table 3).

Table 2 Performance of C57BL/6 mice fed diets supplemented with alanine or leucine (Mean values with their pooled standard errors, n 10)

+Ala, l-alanine-supplemented diet; +Leu, l-leucine-supplemented diet.

Fig. 1 Effects of dietary leucine (Leu) supplementation on plasma leptin concentration (ng/ml) in C57BL/6 mice. Mice were fed the Leu-supplemented diet or the alanine (Ala)-supplemented (isonitrogenous control) diet for 14 d. After the mice received their diets for 2 h on day 14, blood samples were obtained from the orbital sinus. Plasma leptin concentrations were measured. Values are means (n 6), with their standard errors represented by vertical bars. a,bMean values with unlike letters were significantly different (P< 0·05).

Table 3 Amino acid and urea concentrations in the plasma of C57BL/6 mice fed diets supplemented with alanine or leucine (Mean values with their pooled standard errors, n 6)

+Ala, l-alanine-supplemented diet; +Leu, l-leucine-supplemented diet.

Mean values were significantly different from those of the +Ala group: * P< 0·05, ** P< 0·01.

Effect of dietary leucine supplementation on leptin receptor expression and protein metabolism in the skeletal muscles of C57BL/6 mice

Dietary leucine supplementation increased (P< 0·01) the mRNA expression of leptin receptors in the gastrocnemius and soleus muscles (Fig. 2), and also increased (P< 0·01) leptin receptor protein abundance in the gastrocnemius and soleus muscles (Fig. 3). The FSR of the gastrocnemius and soleus muscles in mice fed the leucine-supplemented diet were significantly higher than those in mice fed the alanine-supplemented diet (P< 0·01; Table 4). In addition, dietary leucine supplementation significantly decreased the rate of protein degradation in the gastrocnemius and soleus muscles of C57BL/6 mice (P< 0·05; Table 4).

Fig. 2 Effects of dietary leucine (Leu) supplementation on leptin receptor mRNA expression in skeletal muscles. Mice were fed the Leu-supplemented diet or the alanine (Ala)-supplemented (isonitrogenous control) diet for 14 d. After the mice received their diets for 2 h on day 14, the (A) gastrocnemius and (B) soleus muscles were excised and used for quantitative real-time PCR analysis. The relative abundance for the leptin receptor mRNA was normalised to that for β-actin. Values are means (n 6), with their standard errors represented by vertical bars. a,bMean values with unlike letters were significantly different (P< 0·05).

Fig. 3 Effects of dietary leucine (Leu) supplementation on leptin receptor protein levels in skeletal muscles. Mice were fed the Leu-supplemented diet or the alanine (Ala)-supplemented (isonitrogenous control) diet for 14 d. After the mice received their diets for 2 h on day 14, the (A) gastrocnemius and (B) soleus muscles were excised and used for the Western blot analysis. Representative Western blots are shown and results are expressed as the amount of the leptin receptor relative to β-actin in each group as a percentage of the control. Values are means (n 6), with their standard errors represented by vertical bars. a,bMean values with unlike letters were significantly different (P< 0·05).

Table 4 Fractional synthesis rate and degradation of protein in the gastrocnemius and soleus muscles in C57BL/6 mice fed diets supplemented with alanine or leucine (Mean values with their pooled standard errors, n 6)

+Ala, l-alanine-supplemented diet; +Leu, l-leucine-supplemented diet.

Mean values were significantly different from those of the +Ala group: * P< 0·05, ** P< 0·01.

Effect of leucine and/or leptin treatment on protein metabolism in C2C12 myotubes

Protein synthesis was increased and protein degradation was inhibited in C2C12 myotubes treated with 5 mm-leucine or 50 ng/ml leptin treatment (P< 0·01; Table 5). However, there was no significant difference in the protein synthesis of C2C12 myotubes between the control and leptin-only treatments (P>0·10; Table 5). In addition, there was a significant interaction between the leucine and leptin treatments in regulating protein synthesis (P< 0·05) and degradation (P< 0·01) in C2C12 myotubes (Table 5).

Table 5 Effects of leucine and recombinant mouse leptin treatment on the fractional synthesis rate and degradation of protein in C2C12 myotubes (Mean values with their pooled standard errors, n 6)

− Leptin, no supplemented leptin in medium; +Leptin, leptin-supplemented in medium; − Leu, no supplemented l-leucine in medium; +Leu, l-leucine-supplemented medium.

a,b,cMean values within a row with unlike superscript letters were significantly different (P< 0·05).

Effect of dietary leucine supplementation and/or leptin injection on growth performance and relative weights of the gastrocnemius and soleus muscles in ob/ob mice

Dietary leucine supplementation had no significant effect on the final body weight and feed intake of ob/ob mice (P>0·10; Table 6). Intraperitoneal injection of leptin only decreased the feed intake of ob/ob mice during the first 2 d (P< 0·01; Fig. 4), and tended to decrease the feed intake of ob/ob mice during the whole period of the experiment (P= 0·07; Table 6). In addition, the final body weight of ob/ob mice was significantly reduced by the intraperitoneal injection of leptin (P< 0·01; Table 6). However, there were no significant interactions between dietary leucine supplementation and intraperitoneal leptin injection with regard to the performance of ob/ob mice (P>0·10; Table 6).

Table 6 Effects of dietary leucine supplementation and intraperitoneal leptin injection on performance, relative tissue weights and protein metabolism in the skeletal muscles of ob/ob mice (Mean values with their pooled standard errors, n 6)

− Leptin, intraperitoneal PBS injection; +Leptin, intraperitoneal leptin injection; +Ala, l-alanine-supplemented diet; +Leu, l-leucine-supplemented diet.

a,b,c,dMean values within a row with unlike superscript letters were significantly different (P< 0·05).

Fig. 4 Effects of dietary leucine supplementation and intraperitoneal leptin injection on feed intake in ob/ob mice during 14 d. Ob/ob mice were fed the leucine-supplemented diet or the alanine-supplemented (isonitrogenous control) diet. During 14 d, half of the ob/ob mice on each diet were intraperitoneally injected with sterile PBS or 0·1 μg/g body weight of leptin per d. During 14 d, the feed intake of ob/ob mice was measured per 2 d. Values are means (n 6), with their standard errors represented by vertical bars. * Mean values were significantly different from the alanine+PBS () group (P< 0·05). , Alanine+leptin; , leucine+PBS; , leucine+leptin.

Both dietary leucine supplementation and intraperitoneal leptin injection increased the relative weight of the gastrocnemius and soleus muscles in ob/ob mice (P< 0·01; Table 6). Dietary leucine supplementation and intraperitoneal leptin injection had significant interactions in increasing the relative weight of the gastrocnemius and soleus muscles in ob/ob mice (P< 0·01; Table 6).

Effect of dietary leucine supplementation and/or leptin injection on protein metabolism in ob/ob mice

Both dietary leucine supplementation and intraperitoneal leptin injection stimulated protein synthesis and inhibited protein degradation in the gastrocnemius and soleus muscles of ob/ob mice (P< 0·01; Table 6). In ob/ob mice, there were significant interactions between dietary leucine supplementation and intraperitoneal leptin injection with regard to protein metabolism in the soleus muscles (P< 0·01) but not in the gastrocnemius muscles (P>0·10; Table 6).

Discussion

It has previously been shown that high levels of leucine (>5–6 %) in the standard diet depress feed intake and limit growth in rats and pigs while moderate levels of leucine have no influence on either feed intake or growth(Reference Matsuzaki, Kato and Sakai37Reference Mao, Zeng and Cai39). Moreover, branched-chain amino acids or leucine supplementation in the high-fat diet can decrease the feed intake and growth of rats and mice, but branched-chain amino acids or leucine supplementation in the standard diet do not affect the feed intake and growth of rats and mice(Reference Newgard, An and Bain2, Reference Zhang, Guo and LeBlanc46). In the present study, dietary supplementation with 3 % leucine had no effect on feed intake or weight gain in C57BL/6 or ob/ob mice (Tables 2 and 6). Additionally, intraperitoneal injection of leptin at a concentration of 0·1 μg/g body weight per d for 14 d significantly decreased body weight and feed intake in ob/ob mice during the first 2 d (P< 0·01), but not feed intake in ob/ob mice during the whole period of the experiment (Fig. 4 and Table 6). These results are not consistent with previous studies. Picard et al. (Reference Picard, Richard and Huang40) and Pelleymounter et al. (Reference Pelleymounter, Cullen and Baker41) showed that intraperitoneal injection of leptin with the same dose used in the present experiment significantly decreased feed intake and body weight in ob/ob mice for 7 d when the injection was provided for a 7 d period but not when the treatment lasted for 28 d. Therefore, the difference between the present results and those of others could be due to the differences in the duration of the intraperitoneal injection of leptin. However, Pelleymounter et al. (Reference Pelleymounter, Cullen and Baker41) also showed that the injection dose of 1·0 and 10·0 μg/g body weight of leptin could continuously decrease feed intake and body weight in ob/ob mice for 28 d. These results suggest that when the leptin treatment was provided at a concentration of 0·1 μg/g body weight per d for an extended duration of time, ob/ob mice could have developed leptin resistance, which results in the insignificant effects of leptin injection on feed intake and body weight in the later period of the experiment.

Recent studies have shown that chronic leucine administration can dramatically affect plasma leucine levels(Reference Lynch, Hutson and Patson11, Reference Rieu, Sornet and Bayle47). The present data demonstrated that plasma concentrations of leucine, alanine, glutamate, serine, threonine, tyrosine and valine were significantly altered in mice fed the leucine-supplemented diet compared with mice fed the alanine-supplemented diet (Table 3). In addition, plasma urea concentrations were dramatically lower in leucine-supplemented mice than in the alanine-treated control group (Table 3), which indicates that dietary leucine supplementation may increase the amount of amino acids that are available for tissue growth(Reference Coma, Carrion and Zimmerman48). Previous studies have demonstrated that acute and chronic leucine administration can stimulate protein synthesis and inhibit the protein degradation of skeletal muscles in rats(Reference Combaret, Dardevet and Rieu6, Reference Rieu, Sornet and Bayle47, Reference Suryawan, Jeyapalan and Orellana49, Reference Sugawara, Ito and Nishizawa50). Consistently, the present data indicate that dietary leucine supplementation enhanced protein synthesis and reduced protein degradation in the skeletal muscles of C57BL/6 and ob/ob mice (Tables 4 and 6). In the present study, protein metabolism in the soleus and gastrocnemius muscles was determined. The soleus muscle contains primarily slow-twitch oxidative muscle fibres, but the gastrocnemius muscle contains primarily fast-twitch glycolytic muscle fibres. The results showed that the effect of leucine on protein metabolism in the soleus muscles was larger than that in the gastrocnemius muscles, which could be due to the differences in the type of primary muscle fibres present in these muscles(Reference Escobar, Frank and Suryawan51).

Acute leucine treatment could stimulate the production of specific proteins in various tissues and cells, such as leptin in adipose tissue(Reference Roh, Han and Tzatsos12, Reference Lynch, Gern and Lloyd52Reference Yang, Li and Kong56), while chronic leucine administration has been shown to modestly increase the concentration of plasma leptin in rats(Reference Lynch, Gern and Lloyd52). In the present study, we found that plasma leptin concentrations were dramatically higher in the leucine-supplemented group than those in the alanine-supplemented control group (Fig. 1), which might be due to the dose of leucine in the present study being much higher than that used in previous studies.

Previous studies conducted in our laboratory have shown that leucine promotes leptin receptor expression in mouse C2C12 myotubes through the mammalian target of rapamycin signalling pathway and leptin receptor gene expression(Reference Mao, Zeng and Wang25). Consistent with these findings, the results of the present study demonstrate that dietary leucine supplementation significantly stimulated both mRNA expression and protein levels of leptin receptor in the skeletal muscles of mice (Figs. 2 and 3).

In the present study, we utilised C2C12 myotubes and ob/ob mice as in vitro and in vivo models to study the synergistic effect of leucine and leptin on the protein metabolism of skeletal muscles. C2C12 myotubes, which are generated from the differentiation of C2C12 myoblasts derived from the skeletal muscle of mice, cannot produce or secrete leptin, but can express both the long and short forms of leptin receptor(Reference Berti and Gammeltoft31). In addition, the ob/ob mouse, whose background strain is the C57BL/6J mouse, cannot produce functional leptin on account of a nonsense mutation at the ob gene(Reference Zhang, Proenca and Maffei13). The use of C2C12 myotubes and ob/ob mice may eliminate the effects of endogenous functional leptin on protein metabolism, which also facilitate the investigation of the synergistic effects of leucine and leptin on protein metabolism in skeletal muscles.

Recent reports have shown that leucine and leptin treatments can regulate protein metabolism in skeletal muscles both in vitro and in vivo (Reference Combaret, Dardevet and Rieu6Reference Nakashima, Ishida and Yamazaki8, Reference Carbó, Ribas and Busquets17Reference Lamosová and Zeman19). However, little is known about this synergistic action. In the present study, we found that leucine or leptin treatment stimulated protein synthesis and inhibited protein degradation in the C2C12 myotubes and skeletal muscles of ob/ob mice, which is the reason why dietary leucine supplementation and intraperitoneal leptin injection could increase the relative weight of the gastrocnemius and soleus muscles in ob/ob mice (Tables 5 and 6). These results showed that there was no appearance of leptin resistance during intraperitoneal leptin injection at a concentration of 0·1 μg/g body weight per d for an extended duration of time regulating the muscular protein metabolism of ob/ob mice. In addition, the present results also demonstrate that leucine and leptin treatments had significant interactions in regulating protein synthesis and degradation in the C2C12 myotubes and soleus muscles of ob/ob mice (Tables 5 and 6), but not in the gastrocnemius muscles of ob/ob mice (Table 6). The difference between the soleus and gastrocnemius muscles could be due to the differences in the type of primary muscle fibres present in these muscles. Moreover, previous studies as well as the present study have all demonstrated that leptin can regulate protein metabolism in vivo and in vitro, but there are discrepancies among the results of these studies, which are due to the differences in leptin dose, treatment duration, cell types, animal health status and animal species. Furthermore, in the present study, we found that after leptin injection, protein metabolism in ob/ob mice was still worse than that in C57BL/6 mice, indicating that there are other factors involved in the regulation of protein metabolism in ob/ob mice.

In conclusion, the results of the present study indicate that leptin and leucine synergistically regulate protein metabolism in skeletal muscles both in vivo and in vitro, and that leucine treatment stimulates the expression of leptin receptors in vivo. These findings provide evidence for a possible pathway whereby leucine regulates protein metabolism in skeletal muscles.

Acknowledgements

The present study was financially supported by grants from the National Science Foundation of China (30525029). X. M., X. Z. and S. Q. designed the protocol for these experiments; X. M., X. Z., Z. H. and S. Q. conducted the research; J. W. analysed the data; X. M., X. Z. and S. Q. wrote the paper; S. Q. had the primary responsibility for the final content of the manuscript. None of the authors had conflicts of interest. Special thanks to Professor Philip Thacker from the University of Saskatchewan for editing the manuscript.

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Figure 0

Table 1 Analysed contents of amino acids (g/100 g) in the alanine- and leucine-supplemented non-purified rodent diets

Figure 1

Table 2 Performance of C57BL/6 mice fed diets supplemented with alanine or leucine (Mean values with their pooled standard errors, n 10)

Figure 2

Fig. 1 Effects of dietary leucine (Leu) supplementation on plasma leptin concentration (ng/ml) in C57BL/6 mice. Mice were fed the Leu-supplemented diet or the alanine (Ala)-supplemented (isonitrogenous control) diet for 14 d. After the mice received their diets for 2 h on day 14, blood samples were obtained from the orbital sinus. Plasma leptin concentrations were measured. Values are means (n 6), with their standard errors represented by vertical bars. a,bMean values with unlike letters were significantly different (P< 0·05).

Figure 3

Table 3 Amino acid and urea concentrations in the plasma of C57BL/6 mice fed diets supplemented with alanine or leucine (Mean values with their pooled standard errors, n 6)

Figure 4

Fig. 2 Effects of dietary leucine (Leu) supplementation on leptin receptor mRNA expression in skeletal muscles. Mice were fed the Leu-supplemented diet or the alanine (Ala)-supplemented (isonitrogenous control) diet for 14 d. After the mice received their diets for 2 h on day 14, the (A) gastrocnemius and (B) soleus muscles were excised and used for quantitative real-time PCR analysis. The relative abundance for the leptin receptor mRNA was normalised to that for β-actin. Values are means (n 6), with their standard errors represented by vertical bars. a,bMean values with unlike letters were significantly different (P< 0·05).

Figure 5

Fig. 3 Effects of dietary leucine (Leu) supplementation on leptin receptor protein levels in skeletal muscles. Mice were fed the Leu-supplemented diet or the alanine (Ala)-supplemented (isonitrogenous control) diet for 14 d. After the mice received their diets for 2 h on day 14, the (A) gastrocnemius and (B) soleus muscles were excised and used for the Western blot analysis. Representative Western blots are shown and results are expressed as the amount of the leptin receptor relative to β-actin in each group as a percentage of the control. Values are means (n 6), with their standard errors represented by vertical bars. a,bMean values with unlike letters were significantly different (P< 0·05).

Figure 6

Table 4 Fractional synthesis rate and degradation of protein in the gastrocnemius and soleus muscles in C57BL/6 mice fed diets supplemented with alanine or leucine (Mean values with their pooled standard errors, n 6)

Figure 7

Table 5 Effects of leucine and recombinant mouse leptin treatment on the fractional synthesis rate and degradation of protein in C2C12 myotubes (Mean values with their pooled standard errors, n 6)

Figure 8

Table 6 Effects of dietary leucine supplementation and intraperitoneal leptin injection on performance, relative tissue weights and protein metabolism in the skeletal muscles of ob/ob mice (Mean values with their pooled standard errors, n 6)

Figure 9

Fig. 4 Effects of dietary leucine supplementation and intraperitoneal leptin injection on feed intake in ob/ob mice during 14 d. Ob/ob mice were fed the leucine-supplemented diet or the alanine-supplemented (isonitrogenous control) diet. During 14 d, half of the ob/ob mice on each diet were intraperitoneally injected with sterile PBS or 0·1 μg/g body weight of leptin per d. During 14 d, the feed intake of ob/ob mice was measured per 2 d. Values are means (n 6), with their standard errors represented by vertical bars. * Mean values were significantly different from the alanine+PBS () group (P< 0·05). , Alanine+leptin; , leucine+PBS; , leucine+leptin.