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Protective effects of dietary arginine supplementation against oxidative stress in weaned piglets

Published online by Cambridge University Press:  26 November 2012

Ping Zheng ,
Bing Yu ,
Jun He ,
Gang Tian ,
Yuheng Luo ,
Xiangbing Mao ,
Keying Zhang ,
Lianqiang Che  and
Daiwen Chen
Ping Zheng
Affiliation:
Animal Nutrition Institute, Sichuan Agricultural University, Xinkang Road 46#, Ya'an, Sichuan Province625014, People's Republic of China Animal Disease-Resistance Nutrition Key Laboratory of Sichuan Province, Ya'an625014, People's Republic of China
Bing Yu
Affiliation:
Animal Nutrition Institute, Sichuan Agricultural University, Xinkang Road 46#, Ya'an, Sichuan Province625014, People's Republic of China Animal Disease-Resistance Nutrition Key Laboratory of Sichuan Province, Ya'an625014, People's Republic of China
Jun He
Affiliation:
Animal Nutrition Institute, Sichuan Agricultural University, Xinkang Road 46#, Ya'an, Sichuan Province625014, People's Republic of China Animal Disease-Resistance Nutrition Key Laboratory of Sichuan Province, Ya'an625014, People's Republic of China
Gang Tian
Affiliation:
Animal Nutrition Institute, Sichuan Agricultural University, Xinkang Road 46#, Ya'an, Sichuan Province625014, People's Republic of China Animal Disease-Resistance Nutrition Key Laboratory of Sichuan Province, Ya'an625014, People's Republic of China
Yuheng Luo
Affiliation:
Animal Nutrition Institute, Sichuan Agricultural University, Xinkang Road 46#, Ya'an, Sichuan Province625014, People's Republic of China
Xiangbing Mao
Affiliation:
Animal Nutrition Institute, Sichuan Agricultural University, Xinkang Road 46#, Ya'an, Sichuan Province625014, People's Republic of China Animal Disease-Resistance Nutrition Key Laboratory of Sichuan Province, Ya'an625014, People's Republic of China
Keying Zhang
Affiliation:
Animal Nutrition Institute, Sichuan Agricultural University, Xinkang Road 46#, Ya'an, Sichuan Province625014, People's Republic of China
Lianqiang Che
Affiliation:
Animal Nutrition Institute, Sichuan Agricultural University, Xinkang Road 46#, Ya'an, Sichuan Province625014, People's Republic of China Animal Disease-Resistance Nutrition Key Laboratory of Sichuan Province, Ya'an625014, People's Republic of China
Daiwen Chen*
Affiliation:
Animal Nutrition Institute, Sichuan Agricultural University, Xinkang Road 46#, Ya'an, Sichuan Province625014, People's Republic of China Animal Disease-Resistance Nutrition Key Laboratory of Sichuan Province, Ya'an625014, People's Republic of China
*
*Corresponding author: Professor Daiwen Chen, fax +86 835 2882088, email [email protected]
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Abstract

Oxidative stress is detrimental to animals. Previous studies have indicated that arginine (Arg) may function as a potential substance against oxidative stress. The present study was conducted to explore the potential mechanisms behind the Arg-induced protective effects against oxidative stress in piglets. A total of thirty-six piglets were randomly allocated to six groups with six replicates per group. Piglets were subjected to three dietary treatments (namely two groups per treatment) in week 1 and fed with a basal diet (ArgL) or the basal diet supplemented with 0·8 % (ArgM) or 1·6 % (ArgH) l-Arg, respectively. On day 8, piglets were injected intraperitoneally either with diquat (10 mg/kg body weight) or sterile saline. The whole trial lasted 11 d. Results showed that dietary Arg supplementation did not affect growth performance in week 1. Oxidative stress significantly decreased the growth performance of piglets (P< 0·05). However, ArgH attenuated the negative effects of oxidative stress on feed intake and significantly increased the total antioxidant capacity in the liver under oxidative stress (P< 0·05). Both ArgM and ArgH enhanced the activities of plasma glutathione peroxidases and superoxide dismutases and decreased the IL-6 and TNF-α mRNA level in the liver under oxidative stress (P< 0·05). The present study not only shows that Arg can function as a potential nutrient to alleviate oxidative stress responses through the enhancement of antioxidant capacity, and inhibition of the expression of inflammatory cytokines, but the results also suggest that alleviation of oxidative stress responses using dietary nutrient components deserves further attention in the future.

Keywords

ArginineAntioxidant capacityOxidative stressDiquatWeaned piglets
Type
Full Papers
Information
British Journal of Nutrition , Volume 109 , Issue 12 , 28 June 2013 , pp. 2253 - 2260
Copyright
Copyright © The Authors 2012 

Oxidative stress is an imbalance between the generation of reactive oxygen species (ROS) and the antioxidant defence capacity of the body. Reactive oxygen species, such as superoxide and H2O2(Reference Nappi and Vass1), are constantly generated from oxygen in all aerobic metabolism and pathogenic processes. Under normal circumstances, the ROS in the body are maintained at certain steady-state levels and excessive oxidative radicals are generally eliminated by the antioxidant system including non-enzymic components (for example, glutathione, Se, vitamin E and vitamin C) and a series of antioxidant enzymes (for example, superoxide dismutase (SOD) and glutathione peroxidase (GPx)). For weaned piglets, numerous factors such as environmental factors, weaning and infection can lead to oxidative stress, which may result in growth retardation, disease and even death to piglets.

l-Arginine (Arg), a basic amino acid, serves as an essential precursor for the synthesis of biologically important molecules such as protein, ornithine, proline, polyamines, creatine, NO and agmatine(Reference Wu and Morris2). Traditionally, it has been thought of as a non-essential amino acid. However, it is a nutritionally essential amino acid for young mammals and adults under stress and illness(Reference Wu, Davis and Flynn3). Arg deficiency causes growth retardation, intestinal and reproductive dysfunction, impaired immune and neurological development, cardiovascular and pulmonary abnormalities, impaired wound healing, hyperammonaemia, and even death in animals(Reference Wu, Knabe and Kim4). Our previous study found that oxidative stress depressed the growth performance and decreased the concentration of plasma Arg in weaned piglets(Reference Zheng, Yu and Lv5), indicating that Arg may serve as a limited amino acid under oxidative stress. As previous studies(Reference Suschek, Schnorr and Hemmrich6, Reference Lin, Tsai and Chen7) have indicated that Arg may function as a potential substance against oxidative stress, in the present study, we hypothesised that dietary Arg supplementation could attenuate oxidative stress in piglets. Although many studies have been previously conducted to evaluate the effect of Arg supplementation on oxidative stress in animal models and patients(Reference El-Mesallamy, Abdel Hamid and Gad8, Reference Dasgupta, Hebbel and Kaul9), no studies explored the changes of the antioxidant defence system in weaned piglets after dietary Arg supplementation under oxidative stress. Pro-oxidants such as diquat are widely used to induce oxidative stress in different animal models(Reference Zheng, Yu and Lv5, Reference Fussell, Udasin and Gray10Reference Yumino, Kawakami and Tamura13). The aim of the present study was to evaluate if dietary Arg supplementation could enhance body antioxidative capacity and attenuate diquat-induced oxidative stress in weaned piglets, and offer a theoretical basis for developing Arg as a dietary stress-resistant component in feeds.

Materials and methods

Animals

The experimental procedures followed the actual law of animal protection that was approved by the Animal Care Advisory Committee of Sichuan Agricultural University. All crossbred (Pig Improvement Company; PIC) male piglets weaned at 21 (sem 1) d and housed individually in a stainless-steel cage (1·5 m × 0·7 m × 1·0 m) in a temperature- and humidity-controlled room, maintained at 24–26°C on a 12 h light–dark cycle starting at 08.00 hours. All piglets were given free access to distilled water and feed. Before the formal experiment, all piglets were fed with a basal diet for the start of the experiment of 7 d.

Experimental procedure

A total of thirty-six piglets (8·67 (sem 0·43) kg, 28 (sem 1) d) were allocated to six groups with six replicates per group. Piglets were subjected to three dietary treatments (namely two groups per treatment) in week 1 and fed a basal diet supplemented with varying concentrations of Arg. Diets were as follows: ArgL (basal diet), ArgM (basal diet and supplementation with 0·8 % synthetic l-Arg) and ArgH (basal diet and supplementation with 1·6 % synthetic l-Arg). These diets were formulated according to National Research Council 1998(14) requirements and PIC requirements of practical commercial feed for all nutrients. Ingredients and nutrient composition of the experimental diets are shown in Table 1. All feed was mash. Feed intake was recorded, and feed refusal was collected and weighed daily. Piglets were weighed before the morning meal on days 1, 8 and 12. Average daily feed intake (ADFI), average daily gain (ADG) and the ratio of feed intake:gain (F:G) were calculated. The whole trial lasted for 11 d.

Table 1 Dietary composition and nutrient levels

ArgL, basal diet; ArgM, basal diet and supplementation with 0·8 % synthetic l-arginine; ArgH, basal diet and supplementation with 1·6 % synthetic l-arginine; CP, crude protein.

* A pig fat powder (Beijing AnHaiWei Farm Co. Ltd).

A pig compound enzyme (Wuhan Sunhy Animal Pharmacy Co. Ltd).

An organic compound acidifier ACID LACTM Dry (Kemin Industries, Inc.).

§ The vitamin and mineral premix (maize powder as diluent) provided the following amounts per kg complete diet: retinol, 8·4 mg; cholecalciferol, 0.008 mg; vitamin E, 20 mg; menadione, 1 mg; vitamin B12, 0·03 mg; riboflavin, 5 mg; niacin, 20 mg; pantothenic acid, 15 mg; folic acid, 0·5 mg; thiamin, 1·5 mg; pyridoxine, 2 mg; biotin, 0·1 mg; Fe, 100 mg (FeSO4·7H2O); Cu, 6 mg (CuSO4·5H2O); Zn, 100 mg (ZnSO4·7H2O); Mn, 4 mg (MnSO4.H2O); Se, 0·3 mg (Na2SeO3·5H2O); I, 0·14 mg (KI).

At 08.00 hours on day 8, piglets in each dietary treatment were intraperitoneally injected with diquat at 10 mg/kg body weight or sterile 0·9 % NaCl solution of the same amount, respectively. Diquat (diquat dibromide monohydrate, PS365; Sigma Co.) was dissolved in isotonic saline and filter-sterilised. The concentration of diquat solution was 10 mg/ml.

Before injection (0 h) and at 6, 24, 48 and 96 h post-injection, blood (10 ml per pig) was collected from the portal vein precava into heparinised polyethylene tubes (Axygen Biotechnology Co. Ltd). Plasma was prepared by centrifuging the blood (3000 g, 4°C, 5 min) and immediately stored at − 20°C.

After the blood was collected at 96 h post-injection, piglets were slaughtered by exsanguination according to protocols approved by the Sichuan Agricultural University Animal Care Advisory Committee. Liver samples were removed and snap-frozen in liquid N2 and then stored at − 80°C for assay.

Analytical methods

Measurement of cortisol in plasma

Plasma cortisol concentration was analysed by a commercially available ELISA kit (R&D System). The methods were according to the manufacturer's instructions.

Measurement of enzyme activity

GPx, SOD, total antioxidant capacity (TAC) and concentration of malondialdehyde (MDA) in plasma and liver were measured by assay kits from Nanjing Jiancheng Bioengineering Institute. The methods were according to the manufacturer's instructions.

RNA isolation and reverse transcription

Total RNA was extracted from samples of liver using TRIzol reagent (TaKaRa) according to the manufacturer's instructions. The concentration of RNA in the final preparations was calculated from the optical density at 260 nm. The integrity of RNA was verified by denaturing agarose gel electrophoresis. Reverse transcription was performed using the Prime ScriptTM RT reagent kit (TaKaRa) with a 2 μg RNA sample according to the manufacturer's instructions. The cDNA was used as the template for PCR.

Real-time quantitative PCR

Real-time quantitative PCR was performed in an Option Monitor 3 Real-Time PCR Detection System (Bio-Rad) using the SYBR Green Supermix (TaKaRa). Expression levels of TNF-α and IL-6 in liver were analysed by real-time quantitative PCR with SYBR Green PCR reagents (TaKaRa) and performed by means of the Option DNA Engine (Bio-Rad) using the following cycle parameters: 95°C for 10 s, and forty cycles at 95°C for 5 s and 61°C for 20 s with a final extension at 72°C for 5 min. The gene-specific primers used are listed in Table 2. All primers were purchased from TaKaRa. Fluorescence detection was carried out immediately at the end of each annealing step, and the purity of the amplification was confirmed by analysing the melting curves. Relative gene expression to the housekeeping gene β-actin was performed in order to correct for the variance in amounts of RNA input in the reactions.

Table 2 Primers used for the real-time analyses

Each primer pair used yielded a single peak in the melting curve and a single band with the expected size in agarose gel. The relative gene expressions compared with the housekeeping gene β-actin were calculated using the Pfaffl(Reference Pfaffl15) method.

Statistical analysis

Data before the injection were analysed by one-way ANOVA. Data after the injection were analysed by two-way ANOVA using the general linear model procedure. Model main effects included Arg levels (ArgL, ArgM and ArgH) and oxidative stress (injection of diquat or saline). Probability values of < 0·05 were considered to indicate a significant difference and values between 0·05 and 0·10 to indicate a trend. Variable means for treatments showing significant differences in the ANOVA were separated by Duncan's multiple-range test (P< 0·05). Values were expressed as means with their standard errors. All statistical analysis was performed using SPSS 17.0 (SPSS, Inc.).

Results

Growth performance

The effects of dietary Arg levels and oxidative stress on growth performance of piglets are summarised in Table 3. From day 1 to day 7 (pre-injection), supplementation with Arg did not affect (P>0·10) ADG, ADFI and F:G. From day 8 to day 11 (post-injection), oxidative stress induced by diquat significantly decreased ADG and ADFI (P< 0·05). Supplementation of Arg tended to increase the ADFI of piglets under oxidative stress (P= 0·053). Moreover, ArgH significantly increased ADFI relative to ArgL under oxidative stress (P< 0·05). All piglets subjected to oxidative stress induced by diquat lost weight, so we did not calculate F:G for these groups. Arg × oxidative stress interaction effects did not affect piglet ADG and ADFI.

Table 3 Effects of dietary arginine (Arg) supplementation and diquat injection on growth performance of weaned piglets (Mean values with their standard errors)

SS, injection with sterile saline; OS, oxidative stress (injection with diquat); ArgL, 0·95 % Arg; ArgM, 1·62 % Arg; ArgH, 2·48 % Arg; ADG, average daily gain; ADFI, average daily feed intake; F:G, feed:gain ratio; n/a, not applicable.

* Arg × oxidative stress interaction effect.

Some pigs' weight gain was negative after injection, so not calculated.

Cortisol concentration

As shown in Table 4, supplementation with Arg did not affect the concentration of cortisol before diquat injection. Oxidative stress induced by diquat significantly increased the concentration of cortisol at 48 and 96 h in the ArgL group after injection. ArgM and ArgH significantly decreased the concentration of cortisol at 48 h compared with ArgL under oxidative stress. ArgM significantly decreased the concentration of cortisol at 96 h compared with ArgL under oxidative stress.

Table 4 Effects of dietary arginine supplementation and diquat injection on cortisol concentration in plasma of weaned piglets (ng/ml) (Mean values with their standard errors)

SS, injection with sterile saline; OS, oxidative stress (injection with diquat); ArgL, 0·95 % Arg; ArgM, 1·62 % Arg; ArgH, 2·48 % Arg.

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

* Arg × oxidative stress interaction effect.

Malondialdehyde production and enzyme activities in plasma

Table 5 shows the effect of Arg and diquat on the activity of antioxidant enzymes and MDA in plasma. Supplementation with Arg did not affect the activity of GPx before diquat injection. Oxidative stress induced by diquat significantly decreased the activity of GPx at 6, 24 and 48 h after injection. ArgM or/and ArgH significantly increased the activity of GPx at 6, 48 and 96 h compared with ArgL under oxidative stress. It also can be seen from Table 5 that the activity of GPx in the plasma of piglets had the trend of first decreasing then gradually rising and the activity of GPx was the lowest at 24 h under oxidative stress. Arg × oxidative stress interaction effects had a significant effect on GPx at 6 and 96 h after injection.

Table 5 Effects of dietary arginine supplementation and diquat injection on the activities of antioxidant enzymes and malondialdehyde (MDA) in plasma of weaned piglets (Mean values with their standard errors)

SS, injection with sterile saline; OS, oxidative stress (injection with diquat); ArgL, 0·95 % Arg; ArgM, 1·62 % Arg; ArgH, 2·48 % Arg; GPx, glutathione peroxidase; SOD, superoxide dismutase; TAC, total antioxidant capacity.

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

* Arg × oxidative stress interaction effect.

As shown in Table 5, supplementation of Arg significantly decreased the SOD activity of piglets compared with ArgL before injection. Oxidative stress induced by diquat significantly decreased the activity of SOD at 24 and 48 h after injection. ArgH significantly decreased the activity of SOD at 24 and 96 h after injection with sterile saline. ArgM or/and ArgH significantly increased the activity of SOD at 6, 48 and 96 h compared with ArgL under oxidative stress. It also can be seen from Table 5 that the activity of SOD in plasma of piglets had the trend of first decreasing then gradually rising and the activity of SOD was the lowest at 24 h under oxidative stress. Arg × oxidative stress interaction effects had a significant effect on SOD at 48 and 96 h after injection.

Activity of TAC in plasma was detected (Table 5). Supplementation with Arg did not affect the activity of TAC before diquat injection. Oxidative stress induced by diquat significantly decreased the activity of TAC at 6 h after injection. ArgM or/and ArgH significantly increased the activity of TAC at 6, 24 and 48 h compared with ArgL under oxidative stress. Arg × oxidative stress interaction effects had a significant effect on TAC at 6, 24 and 48 h after injection.

Supplementation with Arg did not affect MDA before diquat injection (Table 5). Oxidative stress induced by diquat significantly increased MDA at 6, 24, 48 and 96 h after injection. ArgM or/and ArgH significantly decreased MDA at 6, 48 and 96 h compared with ArgL under oxidative stress. It also can be seen from Table 5 that the concentration of MDA in the plasma of piglets had the trend of first increasing then gradually decreasing and the concentration of MDA was the highest at 24 h under oxidative stress. Arg × oxidative stress interaction effects had a significant effect on MDA at 6 h after injection.

Malondialdehyde production and enzyme activities in liver

The data for MDA production and enzyme activities in liver are presented in Table 6. Oxidative stress induced by diquat did not affect the activity of GPx in liver (P>0·05). Dietary Arg supplementation significantly increased the activities of GPx in liver under non-oxidative stress and oxidative stress (P< 0·05). Oxidative stress induced by diquat significantly decreased the activity of SOD and TAC in the ArgL group in liver (P< 0·05). ArgM or/and ArgH significantly increased the activities of SOD and TAC in liver under oxidative stress compared with ArgL (P< 0·05). Supplementation of Arg could decrease the concentration of MDA under non-oxidative stress.

Table 6 Effects of dietary arginine supplementation and diquat injection on the activities of antioxidant enzymes and malondialdehyde (MDA) in liver of weaned piglets (Mean values with their standard errors)

SS, injection with sterile saline; OS, oxidative stress (injection with diquat); ArgL, 0·95 % Arg; ArgM, 1·62 % Arg; ArgH, 2·48 % Arg; GPx, glutathione peroxidase; SOD, superoxide dismutase; TAC, total antioxidant capacity.

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

* Arg × oxidative stress interaction effect.

Gene expression

As shown in Fig. 1, ArgM and ArgH significantly decreased IL-6 mRNA level in liver compared with ArgL under non-oxidative stress and oxidative stress. Oxidative stress induced by diquat had no effect on TNF-α mRNA level in liver of the ArgL group (P>0·05). Supplementation with Arg significantly decreased the TNF-α mRNA level in liver under oxidative stress (P< 0·05).

Fig. 1 Effects of dietary arginine (Arg) supplementation and diquat injection on (A) IL-6 and (B) TNF-α mRNA relative expression in liver of weaned piglets. Values are means (n 6), with their standard errors represented by vertical bars. a,b,c,dMean values with unlike letters were significantly different (P< 0·05). ArgL, 0·95 % Arg; ArgM, 1·62 % Arg; ArgH, 2·48 % Arg; OS, oxidative stress (injection with diquat).

Discussion

In livestock production, numerous factors can induce oxidative stress to damage cellular antioxidant defence. Oxidative stress can result in suboptimal health conditions of livestock and a reduction in production efficiency. l-Arg is the key physiological substrate of NO, polyamines, creatine, agmatine, glutamate and proline with enormous biological importance(Reference Montanez, Rodriguez-Caso and Sanchez-Jimenez16, Reference Wu, Bazer and Davis17). Kim & Wu(Reference Kim and Wu18) showed that supplementation of 0·2 and 0·4 % Arg to suckling pigs enhanced ADG by 28 and 66 % between ages 7 and 21 d, respectively. In the present study, dietary Arg supplementation did not affect (P>0·10) ADG, ADFI and F:G before diquat injection. In fact, the effect of Arg supplementation on the performance of piglets is related to the age of piglets, the dose of Arg and the period of supplementation. For example, Hernandez et al. (Reference Hernandez, Hansen and Mullan19) reported that supplementing 0·6 % Arg to a diet containing 1·1 % Arg had no influence on the performance of piglets in the first week after weaning, but significantly increased feed intake and ADG in the third week after weaning.

Oxidative stress significantly decreased ADG and ADFI (P< 0·05), and increased F:G (P< 0·05). This is consistent with previous results that oxidative stress significantly reduced the growth performance of piglets(Reference Yuan, Chen and Zhang20). Arg deficiency may occur under various nutritional and clinical conditions. Accumulating evidence has indicated that Arg levels in plasma are markedly reduced in the sepsis pig model(Reference Luiking, Poeze and Ramsay21). In the present study, supplementation of Arg tended to increase the ADFI of piglets under oxidative stress (P= 0·053), and this is more profound at the high inclusion level of Arg (ArgH). Feed intake of pigs often decreases under stress or injury conditions, and increasing feed intake of pigs under stress conditions helps relieve stress and repair. Our experiment showed that high-Arg supplementation (ArgH) was helpful to piglets under oxidative stress through increasing feed intake. Again, the beneficial effects of dietary Arg supplementation under stress conditions could be widely variable depending on many factors, such as the age of piglets and the level of Arg in the diet. Liu et al. (Reference Liu, Huang and Hou22) reported that dietary supplementation of 0·5 or 1·0 % Arg significantly alleviated weight loss compared with lipopolysaccharide-challenged pigs.

Cortisol, a corticosteroid hormone, is an important physiological effector of homeostasis and commonly used as a biomarker of stress(Reference Kusters, Peppelman and Timmers23). In the present study, oxidative stress significantly increased the concentration of cortisol, and the concentration of MDA in plasma was also increased after diquat injection. MDA which remains after termination of lipid peroxidation provides the basis for the thiobarbituric acid test for measuring lipid peroxidation and products in body fluid(Reference Placer, Cushman and Johnson24). Lipid peroxidation is a biochemical oxidative degradation of unsaturated fatty acids that causes irreversible denaturation of essential proteins. GPx and SOD are two major antioxidant enzymes in mammals, which reduce the accumulation of H2O2 and organic hydroperoxides in the body. The activity of the two enzymes is commonly used to monitor the body's antioxidative capability(Reference Chirino and Pedraza-Chaverri25Reference Coyle, Martinez and Coleman27). In the present study, the activities of the two enzymes in plasma were significantly decreased after diquat injection, suggesting that the antioxidative capabilities of piglets were damaged under oxidative stress. These results are consistent with the findings of Yuan et al. (Reference Yuan, Chen and Zhang20) and Zheng et al. (Reference Zheng, Yu and Lv5). Moreover, we found that dietary supplementation of Arg significantly decreased the concentration of cortisol and MDA, increased the activities of GPx and SOD, and increased the contents of TAC in plasma under oxidative stress. These results indicate that supplementation of Arg can effectively relieve the oxidative stress of piglets. These results are consistent with the findings in the sickle-shaped erythrocyte anaemia model of mice in which supplementation of Arg increased the content of antioxidants in plasma(Reference Dasgupta, Hebbel and Kaul9). Furthermore, we also studied the antioxidant capability of the liver. The results in liver were same as plasma, that supplementation of Arg could significantly increase the activities of GPx, SOD and TAC.

Inflammation is the consequence of oxidative stress, and the pathways that generate the mediators of inflammation, such as adhesion molecules and interleukins, are all induced by oxidative stress. IL-6, a central regulator of inflammatory diseases, is produced at the site of inflammation and plays a key role in the acute-phase response(Reference Dominic28). In the present study, IL-6 mRNA expression in the liver significantly decreased in the ArgL group at 96 h after diquat injection compared with the isotonic saline-injected group. The results from the present study are, however, not consistent with previous findings that oxidative stress increased the concentration of IL-6 in plasma(Reference Furukawa, Fujita and Shimabukuro29). This is probably due to the fact that diquat is removed quickly(Reference Kurisaki and Sato30, Reference Daniel and Gage31). Previous research indicated that when male rats were administered 45 mg/kg diquat dibromide, 95 % of the compound was recovered in urine and faeces in 96 h(32). In the present study, the time we detected the IL-6 mRNA expression change was after 96 h of diquat injection. IL-6 is induced often together with the pro-inflammatory cytokines TNF-α in many alarm conditions(Reference Silverman, Miller and Biron33, Reference Zarkovie, Ignjatovie and Dajak34). Overproduction of pro-inflammatory cytokines has a negative influence on animal health(Reference Mckay and Baird35). In the present study, diquat-induced oxidative stress did not influence TNF-α mRNA expression in liver, and supplementation of Arg could significantly suppress TNF-α mRNA in liver. TNF-α is a cytokine involved in systemic inflammation and can induce inflammation. It is possible that supplementing Arg to pigs attenuates oxidative injury through suppressing the expression of TNF-α. Moreover, IL-6 also plays a crucial role in the regulation of local and systemic acute inflammatory responses by down-regulating the expression of pro-inflammatory cytokines(Reference Gabay36Reference Maggio, Guralnik and Longo38). For instance, IL-6 was shown to inhibit the production of TNF-α, and stimulated the release of soluble TNF-α receptors(Reference Schindler, Mancilla and Endres39). Therefore, the protective effects of Arg on oxidative injury may be attributed in part to the elevated expression of hepatic IL-6, which subsequently decreases the production of the pro-inflammatory cytokine TNF-α.

In conclusion, dietary Arg supplementation significantly alleviates a reduction in feed intake and other negative stress responses in weaned piglets under oxidative stress. The beneficial effects of dietary Arg supplementation are due in part to the enhancement of the total antioxidative capacity, and inhibition of the expression of inflammatory cytokines. Moreover, the present results also suggest that alleviation of the oxidative stress responses using dietary nutrient components, such as Arg, deserves further attention in the future.

Acknowledgements

The authors express their gratitude to the Program for Changjiang Scholars and Innovative Research Team in the University of Ministry of Education of China (no. IRTO555-5) and the earmarked fund for China Agriculture Research System (no. CARS-36) for financial support. P. Z. carried out the study. B. Y. designed the study. J. H. and G. T. assisted in manuscript preparation. L. C., Y. L. and X. M. assisted with all the data analyses. K. Z. and D. C. contributed to the experimental design. There is no conflict of interest to disclose.

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Figure 0

Table 1 Dietary composition and nutrient levels

Figure 1

Table 2 Primers used for the real-time analyses

Figure 2

Table 3 Effects of dietary arginine (Arg) supplementation and diquat injection on growth performance of weaned piglets (Mean values with their standard errors)

Figure 3

Table 4 Effects of dietary arginine supplementation and diquat injection on cortisol concentration in plasma of weaned piglets (ng/ml) (Mean values with their standard errors)

Figure 4

Table 5 Effects of dietary arginine supplementation and diquat injection on the activities of antioxidant enzymes and malondialdehyde (MDA) in plasma of weaned piglets (Mean values with their standard errors)

Figure 5

Table 6 Effects of dietary arginine supplementation and diquat injection on the activities of antioxidant enzymes and malondialdehyde (MDA) in liver of weaned piglets (Mean values with their standard errors)

Figure 6

Fig. 1 Effects of dietary arginine (Arg) supplementation and diquat injection on (A) IL-6 and (B) TNF-α mRNA relative expression in liver of weaned piglets. Values are means (n 6), with their standard errors represented by vertical bars. a,b,c,dMean values with unlike letters were significantly different (P< 0·05). ArgL, 0·95 % Arg; ArgM, 1·62 % Arg; ArgH, 2·48 % Arg; OS, oxidative stress (injection with diquat).