Hostname: page-component-78c5997874-dh8gc Total loading time: 0 Render date: 2024-11-08T01:20:58.694Z Has data issue: false hasContentIssue false
  • English
  • Français

Determination of the anti-inflammatory and cytoprotective effects of l-glutamine and l-alanine, or dipeptide, supplementation in rats submitted to resistance exercise

Published online by Cambridge University Press:  24 May 2016

Raquel Raizel ,
Jaqueline Santos Moreira Leite ,
Thaís Menezes Hypólito ,
Audrey Yule Coqueiro ,
Philip Newsholme ,
Vinicius Fernandes Cruzat  and
Julio Tirapegui
Raquel Raizel*
Affiliation:
Department of Food Science and Experimental Nutrition, Faculty of Pharmaceutical Sciences, University of São Paulo, São Paulo, SP 05508-000, Brazil School of Biomedical Sciences, Faculty of Health Sciences and Curtin Health Innovation Research Institute, Curtin University, WA 6102, Australia
Jaqueline Santos Moreira Leite
Affiliation:
Department of Food Science and Experimental Nutrition, Faculty of Pharmaceutical Sciences, University of São Paulo, São Paulo, SP 05508-000, Brazil
Thaís Menezes Hypólito
Affiliation:
Department of Food Science and Experimental Nutrition, Faculty of Pharmaceutical Sciences, University of São Paulo, São Paulo, SP 05508-000, Brazil
Audrey Yule Coqueiro
Affiliation:
Department of Food Science and Experimental Nutrition, Faculty of Pharmaceutical Sciences, University of São Paulo, São Paulo, SP 05508-000, Brazil
Philip Newsholme
Affiliation:
School of Biomedical Sciences, Faculty of Health Sciences and Curtin Health Innovation Research Institute, Curtin University, WA 6102, Australia
Vinicius Fernandes Cruzat*
Affiliation:
School of Biomedical Sciences, Faculty of Health Sciences and Curtin Health Innovation Research Institute, Curtin University, WA 6102, Australia Department of Physiology and Biophysics, Institute of Biomedical Sciences, University of São Paulo, São Paulo, SP 05508-000, Brazil
Julio Tirapegui
Affiliation:
Department of Food Science and Experimental Nutrition, Faculty of Pharmaceutical Sciences, University of São Paulo, São Paulo, SP 05508-000, Brazil
*
*Corresponding author: R. Raizel, email [email protected]; V. F. Cruzat, email [email protected]
*Corresponding author: R. Raizel, email [email protected]; V. F. Cruzat, email [email protected]
Rights & Permissions [Opens in a new window]

Abstract

We evaluated the effects of chronic oral supplementation with l-glutamine and l-alanine in their free form or as the dipeptide l-alanyl-l-glutamine (DIP) on muscle damage, inflammation and cytoprotection, in rats submitted to progressive resistance exercise (RE). Wistar rats (n 8/group) were submitted to 8-week RE, which consisted of climbing a ladder with progressive loads. In the final 21 d before euthanasia, supplements were delivered in a 4 % solution in drinking water. Glutamine, creatine kinase (CK), lactate dehydrogenase (LDH), TNF-α, specific IL (IL-1β, IL-6 and IL-10) and monocyte chemoattractant protein-1 (MCP-1) levels were evaluated in plasma. The concentrations of glutamine, TNF-α, IL-6 and IL-10, as well as NF-κB activation, were determined in extensor digitorum longus (EDL) skeletal muscle. HSP70 level was assayed in EDL and peripheral blood mononuclear cells (PBMC). RE reduced glutamine concentration in plasma and EDL (P<0·05 v. sedentary group). However, l-glutamine supplements (l-alanine plus l-glutamine (GLN+ALA) and DIP groups) restored glutamine levels in plasma (by 40 and 58 %, respectively) and muscle (by 93 and 105 %, respectively). GLN+ALA and DIP groups also exhibited increased level of HSP70 in EDL and PBMC, consistent with the reduction of NF-κB p65 activation and cytokines in EDL. Muscle protection was also indicated by attenuation in plasma levels of CK, LDH, TNF-α and IL-1β, as well as an increase in IL-6, IL-10 and MCP-1. Our study demonstrates that chronic oral l-glutamine treatment (given with l-alanine or as dipeptide) following progressive RE induces cyprotective effects mediated by HSP70-associated responses to muscle damage and inflammation.

Keywords

l-Alanyl-l-glutamineAlanineResistance exerciseInflammationHeat-shock protein
Type
Full Papers
Information
British Journal of Nutrition , Volume 116 , Issue 3 , 14 August 2016 , pp. 470 - 479
Check for updates
Copyright
Copyright © The Authors 2016 

The most abundant amino acid in the body, glutamine, is considered conditionally essential during stress and plays a key role in the inter-organ N transport( Reference Newsholme, Procopio and Lima 1 ), intermediary metabolism( Reference Brosnan 2 ), cellular redox pathways( Reference Newsholme, Procopio and Lima 1 ), glucose( Reference Stumvoll, Perriello and Meyer 3 ) and glutathione synthesis( Reference Cruzat and Tirapegui 4 ), as well as in several other essential metabolic processes( Reference Newsholme 5 , Reference Singleton, Beckey and Wischmeyer 6 ). Glutamine is also an important modulator of the heat-shock protein (HSP) response, via O-glycosylation and phosphorylation of heat-shock factor 1 (HSF-1)( Reference Singleton and Wischmeyer 7 , Reference Wischmeyer 8 ). HSP, especially the 70-kDa family (HSP72+HSP73), are proteins known as ‘stress response proteins’, as their expression is highly induced by different types of agents and catabolic stimuli, such as oxidative, thermal and metabolic stresses, infection and intense exercise( Reference Senf 9 ). Within the cell, HSP act as molecular chaperones maintaining cellular homoeostasis, protecting against injury and death( Reference Senf 9 ) and modulating inflammatory responses through the NF-κB signalling pathway( Reference Shi, Tu and Tang 10 ). Recently, HSP70 was shown to act as a regulator of the early inflammatory response to muscle injury, because of its role in myofibre regeneration and recovery( Reference Senf, Howard and Ahn 11 ).

In sport and exercise, glutamine supplementation is popular among athletes, as it is considered an important nutrient for immune function and muscle recovery from injury and catabolism( Reference Cruzat, Rogero and Tirapegui 12 ). In fact, glutamine is a critical fuel for immune cell function and proliferation( Reference Newsholme 5 , Reference Curi, De Melo and De Azevedo 13 ), and its major supply is from the skeletal muscle, which indicates a tight relationship between muscle and immune function. However, the efficacy of oral l-glutamine supplementation has raised many questions( Reference Cruzat and Tirapegui 4 , Reference Curi, De Melo and De Azevedo 13 Reference Lagranha, Hirabara and Curi 17 ). As studies in humans and animals have described the extensive intestinal metabolism of dietary glutamine( Reference Stoll and Burrin 18 , Reference Zhou, Wu and Yin 19 ), the dipeptide l-alanyl-l-glutamine (DIP) has been utilised for several clinical( Reference Klassen, Mazariegos and Solomons 20 Reference Lima, Carvalho and Figueiredo 22 ) and sports nutrition studies( Reference Rogero, Tirapegui and Pedrosa 16 , Reference Petry, Cruzat and Heck 23 Reference Furst 25 ) as an alternative delivery form via oral administration. The effectiveness of DIP has been related to the intestinal peptide transporter 1, which facilitates a wide broad of dipeptide and tripeptide absorption( Reference Buyse, Berlioz and Guilmeau 26 , Reference Thamotharan, Bawani and Zhou 27 ). The dipeptide also allows for a supply of more glutamine molecules at the physiological osmolality required for oral solutions( Reference Lima, Carvalho and Figueiredo 22 ).

Studies in animal models subjected to intense and exhaustive aerobic exercise( Reference Cruzat and Tirapegui 4 , Reference Petry, Cruzat and Heck 28 ), or subjected to infection( Reference Cruzat, Bittencourt and Scomazzon 29 , Reference Cruzat, Pantaleao and Donato 30 ), have provided evidence that both DIP and free forms of l-glutamine, along with l-alanine supplementation, improve glutamine availability and mitigate muscle damage and related inflammation. Thus, l-alanine supplementation may be important for glutamine metabolism( Reference Cruzat, Krause and Newsholme 24 , Reference Harris, Hoffman and Allsopp 31 ). Considering that progressive resistance exercise (RE) is a commonly used form of exercise and the rat model can mimic human responses to exercise( Reference Goutianos, Tzioura and Kyparos 32 ), the purpose of the present study was to investigate the effects of chronic oral supplementation with l-glutamine and l-alanine, in their free or DIP forms, on muscle damage and inflammation in rats submitted to RE. We hypothesised that supplements containing l-alanine and l-glutamine could favour glutamine metabolism in skeletal muscle composed of fast-twitch fibres, such as the extensor digitorum longus (EDL), and increase the levels of HSP70 in both active muscle and circulating peripheral blood mononuclear cells (PBMC), attenuating the harmful inflammatory effects of heavy RE.

Methods

Animals

Male Wistar rats (n 40), aged 2 months and weighing 228·78 (sd 2·03) g, were obtained from the animal facility of the Faculty of Pharmaceutical Sciences at University of São Paulo and housed one per cage with free access to water and standard chow (NUVILAB CR1; Nuvital Nutrients), composed of 22 % protein. The animals were kept under a 12 h light–12 h dark cycle (lights on 16.00 hours, lights off 04.00 hours), at a room temperature of 22±2°C and relative humidity of 55±10 %, for 8 weeks. Food intake and body weight were registered three times per week, fluid intake was assessed daily and the final weight was determined before euthanasia.

All animals were allowed to adapt to the laboratory environment for 1 week before the beginning of the experimental protocol. After the adaptation period, the animals were weighed and randomly distributed into five groups (n 8/group): sedentary (SED), trained control (CTRL) and trained supplemented with l-alanine (ALA), l-alanine plus l-glutamine (GLN+ALA) or l-alanyl-l-glutamine (DIP). All procedures were approved by the Ethics Committee for Animal Experimentation of the Faculty of Pharmaceutical Sciences, University of São Paulo, according to the guidelines of the Brazilian College of Animal Experimentation (protocol number: CEUA/FCF/428).

Resistance exercise protocol

The 8-week exercise protocol was adapted from Scheffer et al.( Reference Scheffer, Silva and Tromm 33 ), originally published by Hornberger & Farrar( Reference Hornberger and Farrar 34 ), which consisted of climbing a vertical ladder (1·1×0·18 m, 2 cm grid, 80° inclined) with progressive loads secured to the base of the rats tail. During the adaptation period (2 weeks), all animals were familiarised to the apparatus carrying a load equal to 5 % of the body weight. Then, the load training was progressively increased to 25, 50, 75 and 100 % of the body weight, involving three to six sets of eight repetitions, with 2-min break between sets. Each day of exercise was considered one session, and it was repeated every 48 h.

Three tests of maximum carrying capacity (MCC) were performed to determine exercise performance as follows: after adaptation period (test 1), before supplementation (test 2) and after supplementation (test 3). Briefly, the test protocol consisted of a ladder climb with an initial load of 75 % of body weight, plus an additional 30 g load on each climb until exhaustion, with 2 min of rest period. This procedure was successively repeated and the highest load carried was considered the MCC final result.

Supplementation

Supplements were diluted in the drinking water at a concentration of 4 % (4 g dissolved in a final volume of 100 ml) and offered ad libitum in the last 21 d of the experiment. Administration in the drinking water was selected after technical difficulties in administering daily oral gavages and in an attempt to reduce the stress of manipulation, as well as to increase the frequency of amino acid intake throughout the day( Reference Prada, Hirabara and de Souza 35 ). The total amount of amino acids in each administered supplement was calculated based on the commercial DIP concentration (Dipeptiven®; 20 g of l-alanyl-l-glutamine dissolved in 100 ml of water). Free l-glutamine and free l-alanine were manufactured by Labsynth (Synth), whereas Dipeptiven® was manufactured by Fresenius Kabi S.A. Supplement intake was measured daily.

Plasma parameters and peripheral blood mononuclear cell isolation

Blood lactate was determined during RE training every third session of each training load (25, 50, 75 and 100 % of body weight). Samples were collected from the tail vein into heparinised tubes and assayed in a lactometer, Yellow Spring Instruments (YSI Life Science). A duration of 1 h after the last session of RE, animals were killed by decapitation and blood was immediately collected into heparinized tubes and stored at −80°C.

In this study, we analysed the blood buffy coat composed of PBMC (lymphocytes, monocytes and dendritic cells). For PBMC isolation, fresh blood samples were diluted 1:1 in PBS/EDTA (2 mm) and combined with an equal volume of Ficoll–Hypaque solution (Ficoll 400: F4375 and Hypaque: S4506; Sigma-Aldrich) according to the gradient separation method described in the study by Bøyum et al.( Reference Bøyum, Løvhaug and Tresland 36 ). Then, PBMC were aspirated and suspended on ice-cold radioimmunoprecipitation assay (RIPA) buffer containing protease and phosphatase inhibitors (Cell Signaling Technology).

Plasma activity of creatine kinase (CK) and lactate dehydrogenase (LDH) was determined with a commercial kit (Labtest). IL-1β, IL-6, IL-10, TNF-α and monocyte chemoattractant protein-1 (MCP-1) levels were measured by the Luminex beads assay, using the Milliplex MAP Kit for Luminex 200 reader, according to the manufacturer’s instructions (Millipore Corp.). Glutamine and glutamate concentrations were determined spectrophotometrically using a commercial kit (Sigma-Aldrich) adapted for microplate reader (Synergy H1 Hybrid wavelength; BioTek).

Tissue measurements

EDL skeletal muscle was surgically excised after euthanasia and immediately frozen in liquid N2 for subsequent analysis. Muscle glutamine and glutamate concentrations were determined as described by Lund( Reference Lund 37 ). Mean values were reported as micromoles of glutamine per gram of fresh tissue and as nmol of glutamine/mg of protein. Muscle protein content was quantified using the BCA Protein Assay kit (Pierce; Thermo Scientific). For IL-6, IL-10 and TNF-α analysis, muscle samples (250 mg) were homogenised in 1 ml of PBS buffer containing protease and phosphatase inhibitors, and performed according to the immunoassay kit (Millipore).

Total DNA-binding activity of NF-κB p65 was determined in the nuclear extract of EDL muscle by electrophoretic mobility shift assay. Nuclear fractions were isolated and analysed as per the manufacturer’s instructions using the NF-κB p50/p65 transcription factor assay kit (Abcam). NF-κB p65 was detected at 450 nm. Data were shown as optical density normalised by corresponding nuclear protein concentration, which allows semi-quantitative comparisons of the relative amounts of nuclear NF-κB p65 among groups.

Western blot analysis

After homogenisation with RIPA buffer containing protease and phosphatase inhibitors, EDL skeletal muscle and PBMC lysates were combined with sample buffer containing 240 mm-Tris (pH 6·8), 40 % Glycerol, 0·8 % SDS, 200 mm-β-mercaptoethanol and 0·02 % bromophenol blue. Amounts of protein (40 µg) were subjected to SDS-PAGE and transferred onto nitrocellulose membranes (GE Healthcare).

Membranes were blocked with 0·5 % bovine serum albumin (BSA; Sigma-Aldrich) diluted in PBS with Tween (PBST), washed and incubated at 4°C with gentle shaking overnight, with primary antibody HSP70 1:1000 (Cell Signaling Technology). After three washes, membranes were incubated for 1 h with peroxidase-labelled anti-rabbit IgG antibodies (Cell Signaling Technology) diluted 1:5000 in PBST and 2 % BSA. Blots were visualised on ImageQuant 400 (GE Healthcare) with a 1:1 solution of ECL-Advance Western blotting Reagent (GE Healthcare). Monoclonal anti-β-actin-peroxidase antibody (Sigma-Aldrich) at a ratio of 1:25 000 was used for gel loading control and protein normalisation. The densitometric analysis of the Western blot was performed by the protein level average, normalised to β-actin.

Statistical analysis

Comparisons among groups were carried out by one-way ANOVA with Tukey’s honestly significant differences as a post hoc test. Analyses over multiple time points were performed with repeated measures. Pearson’s correlation coefficient (r) was used as a measure of association. The level of statistical significance was set at P<0·05. Data were analysed using Prism 5.0 for windows and expressed as mean values and standard deviations.

Results

Body weight, food and fluid intake

Body weight gain and food intake were reduced (by 30 and 11 %, respectively) in trained CTRL compared with the SED group (P<0·05). However, no differences were observed among trained groups before the supplementation period (data not shown). As depicted in Table 1, RE training attenuated body weight gain and food intake in CTRL group (P<0·05 v. SED) throughout the supplementation period, and no difference was found in water intake between SED and CTRL groups. Although supplement intake was higher in ALA (65·14 (sd 2·92) ml/d) than in GLN+ALA and DIP groups (60·15 (sd 1·90) and 52·75 (sd 1·90) ml/d, respectively), as well as in all supplemented groups compared with CTRL (P<0·05), l-glutamine or l-alanine administrations did not affect weight gain and food intake.

Table 1 Body weight gain, food and fluid intake of rats submitted to resistance exercise and evaluated during 3-week supplementation periodFootnote § (Mean values and standard deviations; n 8)

SED, sedentary group; CTRL, trained control; ALA, trained supplemented with l-alanine; GLN+ALA, trained supplemented with l-glutamine plus l-alanine in free form; DIP, trained supplemented with l-alanyl-l-glutamine.

* P<0·05 v. SED. † P<0·05 v. CTRL. ‡ P<0·05 v. DIP.

§ SED and CTRL received water and supplements given in a 4 % solution.

Maximum carrying capacity performance test and the lactate response

The MCC test represents a method to determine exercise performance( Reference Hornberger and Farrar 34 ). As depicted in Fig. 1, all trained animals demonstrated increased performance (P<0·05) in tests 2 and 3 (approximately 32 and 50 %, respectively) when compared with the first test. However, it is noteworthy that no difference was observed between test 2 and test 3, which suggests a lower carrying capacity induced by high-intensity RE. Although l-glutamine is expected to be useful to replenish amino acid body stores, it is unlikely that this nutritional supplementation can enhance performance, as previously reported( Reference Gleeson 15 , Reference Nogiec and Kasif 38 , Reference Candow, Chilibeck and Burke 39 ). In fact, the MCC test results demonstrated no significant difference between controls and supplemented animals (Fig. 1).

Fig. 1 Maximum carrying capacity (MCC) test was performed before supplementation (test 1 and test 2) and after supplementation period (test 3) over the course of resistance exercise protocol. Values are means (n 8), and standard deviations. * P<0·05 test 1 v. test 2; ** P<0·01 test 1 v. test 3. , Trained control group; , trained supplemented with l-alanine; , l-alanine plus l-glutamine; , dipeptide l-alanyl-l-glutamine.

Lactate concentration was determined in four different time points to evaluate exercise intensity and metabolic demand. As illustrated in Fig. 2, controls exhibited blood lactate 2-fold higher at a load of 100 % compared with all previous loads (P<0·05), suggesting increased energy demand promoted by RE. In the supplemented groups, lactate at 100 % of BW increased approximately 80 %, which was statistically significant when compared with the 25 % load (P<0·05). Moreover, both l-glutamine-supplemented groups were associated with lower lactate concentration at 100 %, when compared with the controls (P<0·05).

Fig. 2 Levels of blood lactate in rats submitted to progressive resistance training. Lactate was assessed in four time points, every third session of each training load (25, 50, 75 and 100 % of body weight). Trained control group (CTRL, ) received water; ALA (), GLN+ALA () and DIP () were supplemented with l-alanine, l-alanine plus l-glutamine and l-alanyl-l-glutamine, respectively, in a 4 % solution. Values are means (n 8), and standard deviations. * P<0·05 v. 25, 50 and 75 % of BW load; P<0·05 v. 25 % of BW load; P<0·05 GLN+ALA and DIP v. CTRL. ALA, Trained supplemented with l-alanine; GLN+ALA, l-glutamine plus l-alanine; DIP, dipeptide l-alanyl-l-glutamine.

Glutamine metabolism in plasma and skeletal muscle

Because of the increased requirements triggered by heavy exercise training, the concentration of glutamine in plasma and tissues falls sharply, especially in major stores of the amino acid for the whole body, such as the skeletal muscle. The results presented herein demonstrated that RE training compromised both plasma (Table 2) and muscle (Table 3) glutamine levels, and the muscle glutamine:glutamate ratio (Table 3) in the controls, when compared with SED animals (P<0·05). In contrast, the nutritional interventions with ALA, GLN+ALA and DIP reduced the severity of RE effects, increasing plasma glutamine concentration (by 45, 40 and 57 %, respectively), when compared with the CTRL group (P<0·05). Moreover, muscle glutamine concentrations were significantly restored (both μmol/g fresh tissue and nmol/mg protein) in GLN+ALA and DIP groups (Table 3).

Table 2 Glutamine, glutamate and markers of muscle damage and inflammation in plasma of rats submitted to 8-week resistance exerciseFootnote § (Mean values and standard deviations; n 8)

SED, sedentary group; CTRL, trained control; ALA, trained supplemented with l-alanine; GLN+ALA, trained supplemented with l-glutamine plus l-alanine in free form; DIP, trained supplemented with l-alanyl-l-glutamine; CK, creatine kinase; LDH, lactate dehydrogenase; MCP-1, monocyte chemoattractant protein-1.

* P<0·05 v. SED.

P<0·05 v. CTRL.

P<0·05 v. GLN+ALA and DIP.

§ SED and CTRL received water and supplements given in a 4 % solution.

Table 3 Skeletal muscle contents of glutamine and glutamate and inflammation markers of rats submitted to 8-week resistance exerciseFootnote (Mean values and standard deviations; n 8)

SED, sedentary group; CTRL, trained control; ALA, trained supplemented with l-alanine; GLN+ALA, trained supplemented with l-glutamine plus l-alanine in free form; DIP, trained supplemented with l-alanyl-l-glutamine.

* P<0·05 v. SED.† P<0·05 v. CTRL.

SED and CTRL received water and supplements given in a 4 % solution.

Although the amino acid intake was increased in supplemented groups (by 33 %) compared with CTRL, no significant correlation was observed between amino acid intake and the concentrations of glutamine in plasma of ALA (r −0·28, P=0·59), GLN+ALA (r −0·42, P=0·40) and DIP (r −0·40, P=0·42) groups, as well as in muscle (r 0·04, P=0·93; r 0·33, P=0·52; r 0·10, P=0·85, respectively).

Muscle damage and inflammation in plasma and skeletal muscle

Assessing plasma markers of muscle damage involved determination of the activity of CK and LDH. This was high in the controls (56 and 39 %, respectively) as compared with the SED group (Table 2, P<0·05). However, this effect was attenuated by GLN+ALA and DIP supplementation, when compared with the CTRL group (P<0·05).

Besides elevations in CK and LDH, RE increased plasma IL-1β by 75 %, TNF-α by 14 %, IL-6 by 45 %, IL-10 by 46 % and MCP-1 by 33 % in the CTRL group as compared with SED (P<0·05). Nevertheless, nutritional interventions with ALA, GLN+ALA and DIP reduced plasma concentrations of IL-1β and TNF-α (by 57 and 21 %, respectively), when compared with controls (P<0·05). Interestingly, animals supplemented with GLN+ALA and DIP exhibited an increase in the concentration of IL-6 (38 %), IL-10 (91 %) and MCP-1 (28 %), as compared with the CTRL group (Table 2, P<0·05).

As depicted in Table 3, both RE training and nutritional supplementation had an impact on muscle inflammation. In the CTRL group, inflammatory mediators such as TNF-α, IL-6 and IL-10 increased because of the RE training protocol, when compared with SED animals (P<0·05). However, ALA, GLN+ALA and DIP supplements attenuated this finding (P<0·05 v. CTRL group), maintaining the concentration of muscle TNF-α, IL-6 and IL-10 close to basal levels observed in the SED group.

Glutamine effects on HSP70 response and muscle NF-κB activation

HSP, especially the HSP70 family (the major HSP), provide critical protection against several forms of injury. Although exercise is a potent stimulus for the HSP response, local and systemic inflammatory injury leads to a deficit in HSP70 protein levels, which may impair recovery. Herein, muscle HSP70 level was markedly reduced (by 51 %) by RE training in the controls, as compared with SED animals (Fig. 3, P<0·05). Moreover, RE produced a severe decrease (by 88 %) in HSP70 levels in circulating PBMC (Fig. 4, P<0·05) possibly because these cells are unable to synthesise glutamine and are largely dependent on plasma and muscle glutamine availability, which is compromised by RE. In fact, glutamine availability is critical for the optimal regulation of HSP response. Indeed, GLN+ALA and DIP supplements were able to restore HSP70 concentration in both EDL skeletal muscle (Fig. 3) and PBMC (Fig. 4), when compared with CTRL animals (P<0·05).

Fig. 3 HSP70 protein levels in extensor digitorum longus (EDL) muscle of rats submitted to resistance exercise. Sedentary (SED) and trained control (CTRL) groups received water; ALA, GLN+ALA and DIP groups were submitted to 8-week resistance exercise and supplemented with l-alanine, l-alanine plus l-glutamine and l-alanyl-l-glutamine, respectively, in a 4 % solution. Supplements were given ad libitum in the last 21 d of the experiment. EDL muscle was excised and immediately frozen in liquid N2 for further analysis. Homogenates were immunoblotted for HSP70 and bands were normalised with β-actin controls. Values are means (n 8), and standard deviations represented by vertical bars. * P<0·05 v. SED; P<0·05 v. CTRL. ALA, Trained supplemented with l-alanine; GLN+ALA, l-glutamine plus l-alanine; DIP, dipeptide l-alanyl-l-glutamine.

Fig. 4 HSP70 protein levels in peripheral blood mononuclear cells (PBMC) of rats submitted to resistance exercise. Sedentary (SED) and trained control (CTRL) groups received water; ALA, GLN+ALA and DIP groups were submitted to 8-week resistance exercise and supplemented with l-alanine, l-alanine plus l-glutamine and l-alanyl-l-glutamine, respectively, in a 4 % solution. Supplements were given ad libitum in the last 21 d of the experiment. Fresh blood samples were collected and peripheral blood mononuclear cells (PBMC) were separated by Ficoll density gradient centrifugation. Homogenates were immunoblotted for HSP70 and bands normalised with β-actin controls. Values are means (n 8), and standard deviations represented by vertical bars. * P<0·05 v. SED; P<0·05 v. CTRL. ALA, Trained supplemented with l-alanine; GLN+ALA, l-glutamine plus l-alanine; DIP, dipeptide l-alanyl-l-glutamine.

Intracellular HSP70 have important anti-inflammatory properties, providing stress tolerance by blocking the activation of the NF-κB pathway( Reference Cruzat, Pantaleao and Donato 30 , Reference Singleton and Wischmeyer 40 ). Our results with RE training are in agreement with in vitro and aerobic exercise studies, since decreased HSP70 levels promoted inflammatory effects by enhancing the activation of NF-κB p65 in the skeletal muscle of controls by 34 %, as compared with the SED group (Fig. 5, P<0·05). Moreover, glutamine is a key substrate that has an impact on HSP70 expression. Consequently, the increased HSP70 levels found in EDL reduced (by 30 %) NF-κB p65 activation, when compared with controls (P<0·05).

Fig. 5 NF-κB p65 DNA-binding activity in the nuclear extract of extensor digitorum longus muscle of rats submitted to resistance exercise. Sedentary (SED) and trained control (CTRL) groups received water; ALA, GLN+ALA and DIP groups were submitted to 8-week resistance exercise and supplemented with l-alanine, l-alanine plus l-glutamine and l-alanyl-l-glutamine, respectively, in a 4 % solution. Supplements were given ad libitum in the last 21 d of the experiment. EDL muscle was excised and frozen in liquid N2 for further preparation of nuclear extract. Values are means (n 8), and standard deviations represented by vertical bars. *P<0·05 v. SED; P<0·05 v. CTRL. ALA, Trained supplemented with l-alanine; GLN+ALA, l-glutamine plus l-alanine; DIP, dipeptide l-alanyl-l-glutamine.

Discussion

Our study demonstrated that chronic oral l-glutamine treatment (in free form along with l-alanine or as dipeptide) following progressive RE promotes cyprotective effects involving HSP70 responses, thus reducing muscle damage and inflammation. Glutamine is widely accepted as an important amino acid for cell metabolism and function, serving as a key metabolic substrate to provide a fuel source and aid N balance( Reference Stoll and Burrin 18 , Reference Zhou, Wu and Yin 19 ). Glutamine metabolism and blood concentration is dramatically compromised under catabolic situations, which include high intensity and long periods of exercise. Surprisingly, little data exist on glutamine metabolism following exogenous supply in predominantly anaerobic activities, such as RE training.

As described herein, RE resulted in lower glutamine concentrations in plasma and EDL muscle. Muscle tissue is quantitatively the largest biosynthetic source and is essential for glutamine production and release, influencing plasma glutamine concentration, as well as its utilisation by other tissues and cells such as PBMC( Reference Newsholme 5 , Reference Curi, De Melo and De Azevedo 13 , Reference Cruzat, Krause and Newsholme 24 , Reference Santos, Caperuto and Costa Rosa 41 ). Although glutamine accounts for at least 50 % of the free pool of amino acids in skeletal muscle, under catabolic situations the release of glutamine from muscle exceeds synthesis, and it may impair recovery from muscle damage because of the enhanced rate of protein breakdown induced by N imbalance following exercise( Reference Newsholme, Procopio and Lima 1 , Reference Newsholme 5 , Reference Cruzat, Krause and Newsholme 24 ). In the current study, chronic oral administration with l-glutamine and l-alanine, in their free form or as the dipeptide, did not influence food intake and body weight gain, which allowed us to evaluate the exclusive effect of supplements in trained rats. The beneficial effects described here are supportive of results published in other studies( Reference Cruzat and Tirapegui 4 , Reference Cruzat, Rogero and Tirapegui 12 , Reference Rogero, Tirapegui and Pedrosa 16 , Reference Petry, Cruzat and Heck 23 , Reference Cruzat, Bittencourt and Scomazzon 29 ).

Interestingly, l-alanine co-supplementation significantly increased glutamine concentration and effects. Exercise is characterised by a shift in blood flow from the gastrointestinal tract to the active muscle, which may lead to changes in intestinal absorption of glutamine, as demonstrated in catabolic conditions( Reference Zhou, Wu and Yin 19 ). The presence of alanine in supplements containing glutamine has been shown to alter glutamine metabolism, as it is metabolised via alanine aminotransferase to pyruvate, and rapidly consumed in the Krebs Cycle to generate ATP and glutamate production from 2-oxoglutarate( Reference Petry, Cruzat and Heck 23 , Reference Cunningham, McClenaghan and Flatt 42 , Reference Battezzati, Haisch and Brillon 43 ). Similar to glutamine, alanine has a central role for maintenance of intermediary metabolism( Reference Cruzat, Krause and Newsholme 24 ). Elevated alanine release from muscle observed during exercise and following training has been considered necessary to provide a non-toxic form of N transport from muscle and a substrate for gluconeogenesis in the liver, as glycolytic flux is increased proportionally to the work intensity during muscle contractions( Reference Hood and Terjung 44 ). Thus, despite the fact that high energy demand evidenced by blood lactate increases in this study, the high glutamine concentration in plasma of rats treated with l-alanine supports the concept that alanine supplementation may supply extra substrate for liver and kidney gluconeogenesis sparing glutamine. Oral supplementation with glutamine given in combination with other amino acids has beneficial effects on reducing inflammatory cytokine levels( Reference Zhou, Wu and Yin 19 ). Herein, we have described the beneficial effects of l-alanine supplementation by reducing pro-inflammatory cytokines; however, administration of l-alanine alone did not enhance the glutamine content of skeletal muscle of trained rats.

Glutamine has also been used as an enhancer of HSP 70 kDa (HSP70) levels( Reference Petry, Cruzat and Heck 23 , Reference Wischmeyer, Kahana and Wolfson 45 ) via O-glycosylation and phosphorylation of HSF-1( Reference Singleton and Wischmeyer 7 , Reference Wischmeyer 8 ) in both stressed and unstressed animals( Reference Wischmeyer, Kahana and Wolfson 45 ). HSP of 70 kDa (HSP70) is one of the most inducible HSP isoforms and interacts with other proteins in an ATP-dependent manner, induced by various stimuli such as exercise, muscle injury and regeneration( Reference Senf 9 , Reference Milne and Noble 46 ). HSP70 has been considered to play an important role in regulating skeletal muscle plasticity( Reference Petry, Cruzat and Heck 23 , Reference Milne and Noble 46 , Reference Peake, Suzuki and Hordern 47 ), apoptosis and cell death by affecting protein folding, ubiquitin degradation pathways and protein translocation( Reference Takayama, Reed and Homma 48 ). Recently, a chaperone balance hypothesis has been proposed. The activation of NF-κB can result in lower levels of intracellular HSP70, releasing pro-inflammatory extracellular HSP70, which may act to reduce oxidative stress in target cells. However, when chronically elevated, extracellular HSP70 stimulates inflammation, oxidative stress, reduction of HSF-1 expression and eventually reduced intracellular HSP70( Reference Krause, Heck and Bittencourt 49 ).

In order to investigate the heat-shock response following progressive RE training, a common form of exercise, we evaluated HSP70 protein levels in fast-twitch EDL muscle, a type of muscle that can generate high-power outputs during exercise( Reference Barclay, Constable and Gibbs 50 ). Although exercise is known to stimulate the HSP response, we report herein that total HSP70 content in EDL muscle markedly decreased in the CTRL group, which may have been a consequence of impairment of glutamine availability and activation of NF-κB. The suppression of HSP response was also found in PBMC, a critical component of the immune system involved in the muscle repair process after exercise, as these cells are a primary source of pro-inflammatory cytokine release( Reference Risøy, Raastad and Hallén 51 Reference Wischmeyer, Riehm and Singleton 53 ). PBMC are largely dependent on skeletal muscle glutamine synthesis and release into blood, as these cells do not possess glutamine synthetase to catalyse glutamine synthesis from ammonia and glutamate( Reference Gleeson 15 ). Glutamine may directly modulate pro-inflammatory cytokine release in PBMC, which may be related to the heat-shock response( Reference Wischmeyer, Riehm and Singleton 53 ). Herein, treatments with DIP and GLN+ALA evoked a cytoprotective response to damaged tissue mediated by replenishment of glutamine concentrations, besides increased HSP70 levels in skeletal muscle and PBMC.

HSP70 has been considered a regulator of the early inflammatory response to muscle injury because of its beneficial role in myofibre regeneration and recovery( Reference Senf, Howard and Ahn 11 ). The increase of HSP70 results in the inhibition of inflammatory cytokine production in human PBMC( Reference Wischmeyer, Riehm and Singleton 53 ), as well as by inactivation of the NF-κB signalling pathway( Reference Shi, Tu and Tang 10 , Reference Milne and Noble 46 , Reference Pahl 54 ). Our results suggest that HSP70 high levels attenuated the production of inflammatory cytokines by inactivation of NF-κB. Inflammatory responses are mediated by activation of critical signalling pathways, such as NF-κB( Reference Shi, Tu and Tang 10 , Reference Cooper, Radom-Aizik and Schwindt 55 Reference Chen, Shi and Qi 57 ). In a single acute exercise bout, the NF-κB activity in skeletal muscle of rats is increased( Reference Vella, Caldow and Larsen 58 , Reference Ji, Gomez-Cabrera and Steinhafel 59 ). The NF-κB pathway acts as a central integrator of responses to mechanical, oxidative and inflammatory stress( Reference Pahl 54 ). However, continuous activation and production of inflammatory components can stimulate excessive recruitment of immune cells, promoting further tissue injury( Reference Urso 60 ). Our study demonstrated an increase in NF-κB p65 nuclear activity in EDL muscle of CTRL animals. Conversely, all nutritional treatments attenuated the effect of RE. Glutamine can attenuate the activation of multiple pathways of inflammation such as NF-κB through the ubiquitin–proteasome pathway, conferring protection against exacerbated inflammatory conditions( Reference Chen, Shi and Qi 57 , Reference Lesueur, Bôle-Feysot and Bekri 61 ).

A decrease in glutamine levels is well established in stressful situations, such as high intensity and prolonged exercise (resulting in severe damage), as well as activation of inflammatory processes, raising the rate of protein degradation( Reference Stumvoll, Perriello and Meyer 3 , Reference Cruzat and Tirapegui 4 , Reference Cruzat, Rogero and Tirapegui 12 , Reference Curi, De Melo and De Azevedo 13 , Reference Rogero, Tirapegui and Pedrosa 16 , Reference Petry, Cruzat and Heck 23 ). In this study, RE induced an increase in plasma levels of CK and LDH enzymes. Despite the fact that CK and LDH are known as late markers of cellular injury, our exercise protocol was able to promote significant changes in 1 h after the last exercise session. A recent study( Reference Baltusnikas, Venckunas and Kilikevicius 62 ) has demonstrated that eccentric contractions induce a significant increase in muscle CK efflux immediately after exercise. Mechanical contractions produced by RE can induce micro-traumas in muscle fibres promoting breakdown of the extracellular matrix, basal lamina and sarcolemma, which leads to changes in membrane structure and permeability( Reference Cooper, Radom-Aizik and Schwindt 55 ). CK is located almost exclusively in brain, skeletal and cardiac muscle and is released to the bloodstream after damage to the structure of non-contractile muscle elements, which is induced by intense exercise( Reference Finsterer 56 ). Moderate bouts of eccentric exercise can induce physiological muscle adaptation; however, repeated intense exercise may induce higher release of muscle damage markers and loss of muscle proteins( Reference Brentano and Martins Kruel 63 Reference Brancaccio, Limongelli and Maffulli 66 ). This was observed in the CTRL group, which indicates additional muscle damage after each exercise session.

Despite harmful effects of RE training, there was a decline in plasma CK and LDH activity in groups supplemented with glutamine (GLN+ALA; DIP), suggesting that muscle became more resistant to subsequent injury caused by a new session of RE. A recent study showed inhibition of signalling proteins that activate protein degradation after acute RE in rats supplemented with l-alanylglutamine( Reference Wang, Choi and Solares 67 ), and previous studies published by our group indicated that l-glutamine-containing supplements represent an effective way to maintain l-glutamine levels, which results in attenuation of the release of substances indicative of muscle damage and oxidative stress in trained rats( Reference Cruzat and Tirapegui 4 , Reference Cruzat, Rogero and Tirapegui 12 , Reference Petry, Cruzat and Heck 23 ).

The increase of lactate induced by high metabolic demand in RE promotes mobilisation of WBC into the circulation( Reference Risøy, Raastad and Hallén 51 ). Muscle micro-injury also induces an influx of macrophages from the circulation in order to promote muscle repair and remodelling, through production of pro- and anti-inflammatory cytokines( Reference Ihalainen, Walker and Paulsen 52 , Reference Pedersen and Febbraio 68 , Reference Petersen and Pedersen 69 ). However, continuous injuries without adequate rest periods trigger chronic inflammatory responses that can exacerbate the underlying injuries and result in reduced performance and impairment of athlete’s health( Reference Peake, Suzuki and Hordern 47 , Reference Finsterer 56 , Reference Peake, Della Gatta and Suzuki 70 ). Our results demonstrate that RE triggered an inflammatory response comprising stimulation of production of pro- and anti-inflammatory mediators.

A bout of heavy RE triggers a transient inflammatory response stimulating pro- and anti-inflammatory cytokine production( Reference Ihalainen, Walker and Paulsen 52 ). Cytokines play an integrative and regulatory role mediating intercellular communication locally or systemically( Reference Peake, Suzuki and Hordern 47 ). According to our results, the exercise protocol induced inflammation by production of pro-inflammatory molecules IL-1β and TNF-α. Exercise induces robust increase of IL-6 from contracting skeletal muscle, and this myokine stimulates the appearance of anti-inflammatory mediators, such as IL-10, besides inhibiting the production of TNF-α ( Reference Cruzat, Bittencourt and Scomazzon 29 , Reference Ihalainen, Walker and Paulsen 52 , Reference Petersen and Pedersen 69 , Reference Steensberg, Fischer and Keller 71 ). It has been reported that factors other than muscle damage, such as stress hormone secretion, increase plasma concentrations of pro-inflammatory cytokines( Reference Steensberg, Fischer and Keller 71 , Reference Pedersen, Steensberg and Keller 72 ), which may explain the plasma increase of IL-6 in this study. Moreover, the magnitude and profile of cytokine response to the exercise may differ in relation to changes in systemic v. local factors during exercise( Reference Hirose, Nosaka and Newton 64 ).

IL-6 has been considered to have a central role in the cytokine response. Enhanced by muscle contraction, IL-6 release is related to changes in Ca homoeostasis, and mRNA levels of IL-6 in skeletal muscle are increased under conditions of low glycogen( Reference Pedersen and Febbraio 68 , Reference Steensberg, Fischer and Keller 71 ). Nonetheless, the relation between glycogen depletion and cytokine production is not completely clear( Reference Nieman, Zwetsloot and Meaney 73 ). A limitation in the current study is that muscle glycogen depletion was not analysed, and it could provide new insights. The RE protocol used in the present work promoted high metabolic activity indicated by increased lactate and, therefore, higher IL-6 concentration in muscle. Higher levels of IL-6 were also observed in plasma of trained and supplemented rats. Pedersen et al.( Reference Pedersen, Steensberg and Keller 72 ) demonstrated that IL-6 induces lipolysis and acts in a hormone-like manner, thus mobilising extracellular substrates or increasing substrate delivery. Although supplemented groups received more energetic substrate, they were associated with lower weight gain, suggesting lipolytic effects of IL-6. However, lower IL-6 levels were observed in EDL muscle of supplemented groups, thus allowing for use of non-lipid fuel supplies.

After eccentric exercise, IL-10 and MCP-1 are increased in an intensity-dependent manner( Reference Peake, Suzuki and Hordern 47 ) in an attempt to contain the inflammation( Reference Vella, Caldow and Larsen 58 ). Produced by a variety of cell types, MCP-1 recruit monocytes into foci of active inflammation and is required for successful muscle regeneration. Impaired muscle regeneration in MCP-1−/− mice suggests an important role for macrophages and MCP-1 in the tissue reparative processes( Reference Shireman, Contreras-Shannon and Ochoa 74 ). As observed in this study, because of greater metabolic demand and exercise-induced stress, the concentrations of MCP-1 were increased in the CTRL group. Glutamine administration in both forms was effective to raise plasma concentrations of MCP-1, leading to high capacity of cellular protection. In this sense, increased production of anti-inflammatory mediators might limit the production of pro-inflammatory cytokines associated with prolonged damage( Reference Cruzat, Krause and Newsholme 24 , Reference Cruzat, Bittencourt and Scomazzon 29 ).

Taken together, these findings demonstrate that chronic oral supplementations with l-glutamine and l-alanine in their free form or as a dipeptide induce cyprotective effects mediated by HSP70 responses, following experimental progressive RE and attenuate harmful and inflammatory effects of RE. l-Glutamine-containing supplements enhanced glutamine availability in plasma and skeletal muscle, which may have stimulated HSP70 higher levels in PBMC and EDL muscle, and reduced DNA-binding activity of NF-kB, supressing inflammation and muscle damage induced by heavy RE.

Acknowledgements

This work was supported by the São Paulo State Foundation for Research (FAPESP, no. 2012/21087-4 and V. F. C. 2015/00446-4), the Brazilian National Council for Scientific and Technological Development (R. R. sandwich doctorate scholarship, no. 233505/2014-8) and the Higher Education and Training Coordination (CAPES).

The present work was designed by R. R., V. F. C. and J. T.; initial manuscript preparation and drafts were prepared by R. R. and revised by V. F. C.; experimental procedures were conducted by R. R., J. S. M. L., T. M. H., A. Y. C.; biochemical and statistical analyses were performed by R. R. and revised by V. F. C.; the final manuscript version was revised by J. T. and P. N.

The authors declare that there are no conflicts of interest.

References

1. Newsholme, P, Procopio, J, Lima, MM, et al. (2003) Glutamine and glutamate – their central role in cell metabolism and function. Cell Biochem Funct 21, 19.CrossRefGoogle ScholarPubMed
2. Brosnan, JT (2001) Amino acids, then and now – a reflection on Sir Hans Krebs’ contribution to nitrogen metabolism. IUBMB Life 52, 265270.CrossRefGoogle Scholar
3. Stumvoll, M, Perriello, G, Meyer, C, et al. (1999) Role of glutamine in human carbohydrate metabolism in kidney and other tissues. Kidney Int 55, 778792.CrossRefGoogle ScholarPubMed
4. Cruzat, VF & Tirapegui, J (2009) Effects of oral supplementation with glutamine and alanyl-glutamine on glutamine, glutamate, and glutathione status in trained rats and subjected to long-duration exercise. Nutrition 25, 428435.CrossRefGoogle ScholarPubMed
5. Newsholme, P (2001) Why is l-glutamine metabolism important to cells of the immune system in health, postinjury, surgery or infection? J Nutr 131, 2515S2522S; discussion 2523S–2514S.CrossRefGoogle ScholarPubMed
6. Singleton, KD, Beckey, VE & Wischmeyer, PE (2005) Glutamine prevents activation of nf-kappab and stress kinase pathways, attenuates inflammatory cytokine release, and prevents acute respiratory distress syndrome (ards) following sepsis. Shock 24, 583589.CrossRefGoogle ScholarPubMed
7. Singleton, KD & Wischmeyer, PE (2008) Glutamine induces heat shock protein expression via O-glycosylation and phosphorylation of HSF-1 and Sp1. JPEN J Parenter Enteral Nutr 32, 371376.CrossRefGoogle ScholarPubMed
8. Wischmeyer, PE (2002) Glutamine and heat shock protein expression. Nutrition 18, 225228.CrossRefGoogle ScholarPubMed
9. Senf, SM (2013) Skeletal muscle heat shock protein 70: diverse functions and therapeutic potential for wasting disorders. Front Physiol 4, 330.CrossRefGoogle ScholarPubMed
10. Shi, Y, Tu, Z, Tang, D, et al. (2006) The inhibition of LPS-induced production of inflammatory cytokines by HSP70 involves inactivation of the NF-kappaB pathway but not the MAPK pathways. Shock 26, 277284.CrossRefGoogle Scholar
11. Senf, SM, Howard, TM, Ahn, B, et al. (2013) Loss of the inducible Hsp70 delays the inflammatory response to skeletal muscle injury and severely impairs muscle regeneration. PLOS ONE 8, e62687.CrossRefGoogle ScholarPubMed
12. Cruzat, VF, Rogero, MM & Tirapegui, J (2010) Effects of supplementation with free glutamine and the dipeptide alanyl-glutamine on parameters of muscle damage and inflammation in rats submitted to prolonged exercise. Cell Biochem Funct 28, 2430.CrossRefGoogle ScholarPubMed
13. Curi, TC, De Melo, MP, De Azevedo, RB, et al. (1997) Glutamine utilization by rat neutrophils: presence of phosphate-dependent glutaminase. Am J Physiol 273, C1124C1129.CrossRefGoogle ScholarPubMed
14. Shewchuk, LD, Baracos, VE & Field, CJ (1997) Dietary l-glutamine does not improve lymphocyte metabolism or function in exercise-trained rats. Med Sci Sports Exerc 29, 474481.CrossRefGoogle ScholarPubMed
15. Gleeson, M (2008) Dosing and efficacy of glutamine supplementation in human exercise and sport training. J Nutr 138, 2045S2049S.CrossRefGoogle ScholarPubMed
16. Rogero, MM, Tirapegui, J, Pedrosa, RG, et al. (2006) Effect of alanyl-glutamine supplementation on plasma and tissue glutamine concentrations in rats submitted to exhaustive exercise. Nutrition 22, 564571.CrossRefGoogle ScholarPubMed
17. Lagranha, CJ, Hirabara, SM, Curi, R, et al. (2007) Glutamine supplementation prevents exercise-induced neutrophil apoptosis and reduces p38 MAPK and JNK phosphorylation and p53 and caspase 3 expression. Cell Biochem Funct 25, 563569.CrossRefGoogle ScholarPubMed
18. Stoll, B & Burrin, DG (2006) Measuring splanchnic amino acid metabolism in vivo using stable isotopic tracers. J Anim Sci 84, Suppl., E60E72.CrossRefGoogle ScholarPubMed
19. Zhou, X, Wu, X, Yin, Y, et al. (2012) Preventive oral supplementation with glutamine and arginine has beneficial effects on the intestinal mucosa and inflammatory cytokines in endotoxemic rats. Amino Acids 43, 813821.CrossRefGoogle ScholarPubMed
20. Klassen, P, Mazariegos, M, Solomons, NW, et al. (2000) The pharmacokinetic responses of humans to 20 g of alanyl-glutamine dipeptide differ with the dosing protocol but not with gastric acidity or in patients with acute Dengue fever. J Nutr 130, 177182.CrossRefGoogle ScholarPubMed
21. Rooyackers, OE, Soeters, PB, Saris, WH, et al. (1995) Effect of an enterally administered glutamine-rich protein on the catabolic response to a zymosan challenge in rats. Clin Nutr 14, 105115.CrossRefGoogle ScholarPubMed
22. Lima, AA, Carvalho, GH, Figueiredo, AA, et al. (2002) Effects of an alanyl-glutamine-based oral rehydration and nutrition therapy solution on electrolyte and water absorption in a rat model of secretory diarrhea induced by cholera toxin. Nutrition 18, 458462.CrossRefGoogle Scholar
23. Petry, ER, Cruzat, VF, Heck, TG, et al. (2014) Alanyl-glutamine and glutamine plus alanine supplements improve skeletal redox status in trained rats: involvement of heat shock protein pathways. Life Sci 94, 130136.CrossRefGoogle ScholarPubMed
24. Cruzat, VF, Krause, M & Newsholme, P (2014) Amino acid supplementation and impact on immune function in the context of exercise. J Int Soc Sports Nutr 11, 61.CrossRefGoogle ScholarPubMed
25. Furst, P (2001) New developments in glutamine delivery. J Nutr 131, 2562S2568S.CrossRefGoogle ScholarPubMed
26. Buyse, M, Berlioz, F, Guilmeau, S, et al. (2001) PepT1-mediated epithelial transport of dipeptides and cephalexin is enhanced by luminal leptin in the small intestine. J Clin Invest 108, 14831494.CrossRefGoogle ScholarPubMed
27. Thamotharan, M, Bawani, SZ, Zhou, X, et al. (1998) Mechanism of dipeptide stimulation of its own transport in a human intestinal cell line. Proc Assoc Am Physicians 110, 361368.Google Scholar
28. Petry, ER, Cruzat, VF, Heck, TG, et al. (2015) l-Glutamine supplementations enhance liver glutamine-glutathione axis and heat shock factor-1 expression in endurance-exercise trained rats. Int J Sport Nutr Exerc Metab 25, 188197.CrossRefGoogle ScholarPubMed
29. Cruzat, VF, Bittencourt, A, Scomazzon, SP, et al. (2014) Oral free and dipeptide forms of glutamine supplementation attenuate oxidative stress and inflammation induced by endotoxemia. Nutrition 30, 602611.CrossRefGoogle ScholarPubMed
30. Cruzat, VF, Pantaleao, LC, Donato, J Jr, et al. (2014) Oral supplementations with free and dipeptide forms of l-glutamine in endotoxemic mice: effects on muscle glutamine-glutathione axis and heat shock proteins. J Nutr Biochem 25, 345352.CrossRefGoogle ScholarPubMed
31. Harris, RC, Hoffman, JR, Allsopp, A, et al. (2012) l-Glutamine absorption is enhanced after ingestion of l-alanylglutamine compared with the free amino acid or wheat protein. Nutr Res 32, 272277.CrossRefGoogle ScholarPubMed
32. Goutianos, G, Tzioura, A, Kyparos, A, et al. (2015) The rat adequately reflects human responses to exercise in blood biochemical profile: a comparative study. Physiol Rep 3, e12293.CrossRefGoogle ScholarPubMed
33. Scheffer, DL, Silva, LA, Tromm, CB, et al. (2012) Impact of different resistance training protocols on muscular oxidative stress parameters. Appl Physiol Nutr Metab 37, 12391246.CrossRefGoogle ScholarPubMed
34. Hornberger, TA & Farrar, RP (2004) Physiological hypertrophy of the FHL muscle following 8 weeks of progressive resistance exercise in the rat. Can J Appl Physiol 29, 1631.CrossRefGoogle ScholarPubMed
35. Prada, PO, Hirabara, SM, de Souza, CT, et al. (2007) l-Glutamine supplementation induces insulin resistance in adipose tissue and improves insulin signalling in liver and muscle of rats with diet-induced obesity. Diabetologia 50, 19491959.CrossRefGoogle ScholarPubMed
36. Bøyum, A, Løvhaug, D, Tresland, L, et al. (1991) Separation of leucocytes: improved cell purity by fine adjustments of gradient medium density and osmolality. Scand J Immunol 34, 697712.CrossRefGoogle ScholarPubMed
37. Lund, P (1970) A radiochemical assay for glutamine synthetase, and activity of the enzyme in rat tissues. Biochem J 118, 3539.CrossRefGoogle ScholarPubMed
38. Nogiec, CD & Kasif, S (2013) To supplement or not to supplement: a metabolic network framework for human nutritional supplements. PLOS ONE 8, e68751.CrossRefGoogle ScholarPubMed
39. Candow, DG, Chilibeck, PD, Burke, DG, et al. (2001) Effect of glutamine supplementation combined with resistance training in young adults. Eur J Appl Physiol 86, 142149.CrossRefGoogle ScholarPubMed
40. Singleton, KD & Wischmeyer, PE (2007) Glutamine’s protection against sepsis and lung injury is dependent on heat shock protein 70 expression. Am J Physiol Regul Integr Comp Physiol 292, R1839R1845.CrossRefGoogle ScholarPubMed
41. Santos, RV, Caperuto, EC & Costa Rosa, LF (2007) Effects of acute exhaustive physical exercise upon glutamine metabolism of lymphocytes from trained rats. Life Sci 80, 573578.CrossRefGoogle ScholarPubMed
42. Cunningham, GA, McClenaghan, NH, Flatt, PR, et al. (2005) l-Alanine induces changes in metabolic and signal transduction gene expression in a clonal rat pancreatic beta-cell line and protects from pro-inflammatory cytokine-induced apoptosis. Clin Sci (Lond) 109, 447455.CrossRefGoogle Scholar
43. Battezzati, A, Haisch, M, Brillon, DJ, et al. (1999) Splanchnic utilization of enteral alanine in humans. Metabolism 48, 915921.CrossRefGoogle ScholarPubMed
44. Hood, DA & Terjung, RL (1994) Endurance training alters alanine and glutamine release from muscle during contractions. FEBS Lett 340, 287290.CrossRefGoogle ScholarPubMed
45. Wischmeyer, PE, Kahana, M, Wolfson, R, et al. (2001) Glutamine induces heat shock protein and protects against endotoxin shock in the rat. J Appl Physiol (1985) 90, 24032410.CrossRefGoogle ScholarPubMed
46. Milne, KJ & Noble, EG (2008) Response of the myocardium to exercise: sex-specific regulation of hsp70. Med Sci Sports Exerc 40, 655663.CrossRefGoogle ScholarPubMed
47. Peake, JM, Suzuki, K, Hordern, M, et al. (2005) Plasma cytokine changes in relation to exercise intensity and muscle damage. Eur J Appl Physiol 95, 514521.CrossRefGoogle ScholarPubMed
48. Takayama, S, Reed, JC & Homma, S (2003) Heat-shock proteins as regulators of apoptosis. Oncogene 22, 90419047.CrossRefGoogle ScholarPubMed
49. Krause, M, Heck, TG, Bittencourt, A, et al. (2015) The chaperone balance hypothesis: the importance of the extracellular to intracellular HSP70 ratio to inflammation-driven type 2 diabetes, the effect of exercise, and the implications for clinical management. Mediators Inflamm 2015, 249205.CrossRefGoogle ScholarPubMed
50. Barclay, CJ, Constable, JK & Gibbs, CL (1993) Energetics of fast- and slow-twitch muscles of the mouse. J Physiol 472, 6180.CrossRefGoogle ScholarPubMed
51. Risøy, BA, Raastad, T, Hallén, J, et al. (2003) Delayed leukocytosis after hard strength and endurance exercise: aspects of regulatory mechanisms. BMC Physiol 3, 14.CrossRefGoogle ScholarPubMed
52. Ihalainen, J, Walker, S, Paulsen, G, et al. (2014) Acute leukocyte, cytokine and adipocytokine responses to maximal and hypertrophic resistance exercise bouts. Eur J Appl Physiol 114, 26072616.CrossRefGoogle ScholarPubMed
53. Wischmeyer, PE, Riehm, J, Singleton, KD, et al. (2003) Glutamine attenuates tumor necrosis factor-alpha release and enhances heat shock protein 72 in human peripheral blood mononuclear cells. Nutrition 19, 16.CrossRefGoogle ScholarPubMed
54. Pahl, HL (1999) Activators and target genes of Rel/NF-kappaB transcription factors. Oncogene 18, 68536866.CrossRefGoogle ScholarPubMed
55. Cooper, DM, Radom-Aizik, S, Schwindt, C, et al. (2007) Dangerous exercise: lessons learned from dysregulated inflammatory responses to physical activity. J Appl Physiol (1985) 103, 700709.CrossRefGoogle ScholarPubMed
56. Finsterer, J (2012) Biomarkers of peripheral muscle fatigue during exercise. BMC Musculoskelet Disord 13, 218.CrossRefGoogle ScholarPubMed
57. Chen, G, Shi, J, Qi, M, et al. (2008) Glutamine decreases intestinal nuclear factor kappa B activity and pro-inflammatory cytokine expression after traumatic brain injury in rats. Inflamm Res 57, 5764.CrossRefGoogle ScholarPubMed
58. Vella, L, Caldow, MK, Larsen, AE, et al. (2012) Resistance exercise increases NF-κB activity in human skeletal muscle. Am J Physiol Regul Integr Comp Physiol 302, R667R673.CrossRefGoogle ScholarPubMed
59. Ji, LL, Gomez-Cabrera, MC, Steinhafel, N, et al. (2004) Acute exercise activates nuclear factor (NF)-kappaB signaling pathway in rat skeletal muscle. FASEB J 18, 14991506.CrossRefGoogle ScholarPubMed
60. Urso, ML (2013) Anti-inflammatory interventions and skeletal muscle injury: benefit or detriment? J Appl Physiol (1985) 115, 920928.CrossRefGoogle ScholarPubMed
61. Lesueur, C, Bôle-Feysot, C, Bekri, S, et al. (2012) Glutamine induces nuclear degradation of the NF-κB p65 subunit in Caco-2/TC7 cells. Biochimie 94, 806815.CrossRefGoogle ScholarPubMed
62. Baltusnikas, J, Venckunas, T, Kilikevicius, A, et al. (2015) Efflux of creatine kinase from isolated soleus muscle depends on age, sex and type of exercise in mice. J Sports Sci Med 14, 379385.Google ScholarPubMed
63. Brentano, MA & Martins Kruel, LF (2011) A review on strength exercise-induced muscle damage: applications, adaptation mechanisms and limitations. J Sports Med Phys Fitness 51, 110.Google ScholarPubMed
64. Hirose, L, Nosaka, K, Newton, M, et al. (2004) Changes in inflammatory mediators following eccentric exercise of the elbow flexors. Exerc Immunol Rev 10, 7590.Google ScholarPubMed
65. Brancaccio, P, Maffulli, N, Buonauro, R, et al. (2008) Serum enzyme monitoring in sports medicine. Clin Sports Med 27, 118 vii.CrossRefGoogle ScholarPubMed
66. Brancaccio, P, Limongelli, FM & Maffulli, N (2006) Monitoring of serum enzymes in sport. Br J Sports Med 40, 9697.CrossRefGoogle ScholarPubMed
67. Wang, W, Choi, RH, Solares, GJ, et al. (2015) l-Alanylglutamine inhibits signaling proteins that activate protein degradation, but does not affect proteins that activate protein synthesis after an acute resistance exercise. Amino Acids 47, 13891398.CrossRefGoogle Scholar
68. Pedersen, BK & Febbraio, MA (2008) Muscle as an endocrine organ: focus on muscle-derived interleukin-6. Physiol Rev 88, 13791406.CrossRefGoogle ScholarPubMed
69. Petersen, AM & Pedersen, BK (2005) The anti-inflammatory effect of exercise. J Appl Physiol (1985) 98, 11541162.CrossRefGoogle ScholarPubMed
70. Peake, JM, Della Gatta, P, Suzuki, K, et al. (2015) Cytokine expression and secretion by skeletal muscle cells: regulatory mechanisms and exercise effects. Exerc Immunol Rev 21, 825.Google ScholarPubMed
71. Steensberg, A, Fischer, CP, Keller, C, et al. (2003) IL-6 enhances plasma IL-1ra, IL-10, and cortisol in humans. Am J Physiol Endocrinol Metab 285, E433E437.CrossRefGoogle ScholarPubMed
72. Pedersen, BK, Steensberg, A, Keller, P, et al. (2003) Muscle-derived interleukin-6: lipolytic, anti-inflammatory and immune regulatory effects. Pflugers Arch 446, 916.CrossRefGoogle ScholarPubMed
73. Nieman, DC, Zwetsloot, KA, Meaney, MP, et al. (2015) Post-exercise skeletal muscle glycogen related to plasma cytokines and muscle IL-6 protein content, but not muscle cytokine mRNA expression. Front Nutr 2, 27.CrossRefGoogle Scholar
74. Shireman, PK, Contreras-Shannon, V, Ochoa, O, et al. (2007) MCP-1 deficiency causes altered inflammation with impaired skeletal muscle regeneration. J Leukoc Biol 81, 775785.CrossRefGoogle ScholarPubMed
Figure 0

Table 1 Body weight gain, food and fluid intake of rats submitted to resistance exercise and evaluated during 3-week supplementation period§ (Mean values and standard deviations; n 8)

Figure 1

Fig. 1 Maximum carrying capacity (MCC) test was performed before supplementation (test 1 and test 2) and after supplementation period (test 3) over the course of resistance exercise protocol. Values are means (n 8), and standard deviations. * P<0·05 test 1 v. test 2; ** P<0·01 test 1 v. test 3. , Trained control group; , trained supplemented with l-alanine; , l-alanine plus l-glutamine; , dipeptide l-alanyl-l-glutamine.

Figure 2

Fig. 2 Levels of blood lactate in rats submitted to progressive resistance training. Lactate was assessed in four time points, every third session of each training load (25, 50, 75 and 100 % of body weight). Trained control group (CTRL, ) received water; ALA (), GLN+ALA () and DIP () were supplemented with l-alanine, l-alanine plus l-glutamine and l-alanyl-l-glutamine, respectively, in a 4 % solution. Values are means (n 8), and standard deviations. * P<0·05 v. 25, 50 and 75 % of BW load; P<0·05 v. 25 % of BW load; P<0·05 GLN+ALA and DIP v. CTRL. ALA, Trained supplemented with l-alanine; GLN+ALA, l-glutamine plus l-alanine; DIP, dipeptide l-alanyl-l-glutamine.

Figure 3

Table 2 Glutamine, glutamate and markers of muscle damage and inflammation in plasma of rats submitted to 8-week resistance exercise§ (Mean values and standard deviations; n 8)

Figure 4

Table 3 Skeletal muscle contents of glutamine and glutamate and inflammation markers of rats submitted to 8-week resistance exercise‡ (Mean values and standard deviations; n 8)

Figure 5

Fig. 3 HSP70 protein levels in extensor digitorum longus (EDL) muscle of rats submitted to resistance exercise. Sedentary (SED) and trained control (CTRL) groups received water; ALA, GLN+ALA and DIP groups were submitted to 8-week resistance exercise and supplemented with l-alanine, l-alanine plus l-glutamine and l-alanyl-l-glutamine, respectively, in a 4 % solution. Supplements were given ad libitum in the last 21 d of the experiment. EDL muscle was excised and immediately frozen in liquid N2 for further analysis. Homogenates were immunoblotted for HSP70 and bands were normalised with β-actin controls. Values are means (n 8), and standard deviations represented by vertical bars. * P<0·05 v. SED; P<0·05 v. CTRL. ALA, Trained supplemented with l-alanine; GLN+ALA, l-glutamine plus l-alanine; DIP, dipeptide l-alanyl-l-glutamine.

Figure 6

Fig. 4 HSP70 protein levels in peripheral blood mononuclear cells (PBMC) of rats submitted to resistance exercise. Sedentary (SED) and trained control (CTRL) groups received water; ALA, GLN+ALA and DIP groups were submitted to 8-week resistance exercise and supplemented with l-alanine, l-alanine plus l-glutamine and l-alanyl-l-glutamine, respectively, in a 4 % solution. Supplements were given ad libitum in the last 21 d of the experiment. Fresh blood samples were collected and peripheral blood mononuclear cells (PBMC) were separated by Ficoll density gradient centrifugation. Homogenates were immunoblotted for HSP70 and bands normalised with β-actin controls. Values are means (n 8), and standard deviations represented by vertical bars. * P<0·05 v. SED; P<0·05 v. CTRL. ALA, Trained supplemented with l-alanine; GLN+ALA, l-glutamine plus l-alanine; DIP, dipeptide l-alanyl-l-glutamine.

Figure 7

Fig. 5 NF-κB p65 DNA-binding activity in the nuclear extract of extensor digitorum longus muscle of rats submitted to resistance exercise. Sedentary (SED) and trained control (CTRL) groups received water; ALA, GLN+ALA and DIP groups were submitted to 8-week resistance exercise and supplemented with l-alanine, l-alanine plus l-glutamine and l-alanyl-l-glutamine, respectively, in a 4 % solution. Supplements were given ad libitum in the last 21 d of the experiment. EDL muscle was excised and frozen in liquid N2 for further preparation of nuclear extract. Values are means (n 8), and standard deviations represented by vertical bars. *P<0·05 v. SED; P<0·05 v. CTRL. ALA, Trained supplemented with l-alanine; GLN+ALA, l-glutamine plus l-alanine; DIP, dipeptide l-alanyl-l-glutamine.