Animals and treatments

The experiment was approved by the Animal Experimental Committee of Wageningen UR Livestock Research. A total of sixteen barrows (Dutch Landrace × York) with an initial BW of 28·5 (sem 0·5) kg were individually housed in metabolism cages (1·3 × 1·3 m) at a room temperature ranging between 18 and 22°C. Based on litter weight and BW, pigs were allocated to one of two treatment groups receiving either an adequate (Ad) or restricted (Res, 70 % of Ad) dietary protein supply at a similar daily supply of other nutrients. To this end, a basal mixture was designed without protein sources. The Ad diet included the basal mixture with the additional protein sources casein, wheat gluten meal, soya protein isolate and potato protein, and met the requirements for essential AA for growing pigs in the range of 35–45 kg BW^{( 25 )} (Table 1). The Res diet included the basal mixture to which 70 % of the quantities of additional protein sources (casein, wheat gluten meal, soya protein isolate and potato protein) were added compared with the quantities included in the Ad diet. In order to supply all pigs with the same amount of the basal mixture, relative to their metabolic BW, the feed allowance of pigs assigned to the Res diet was 94·3 % of that of pigs receiving the Ad diet. The experimental diets were provided in mash form and mixed with water using a feed:water ratio of 1:3. The pigs were fed at 07.00 and 15.30 hours in equal amounts at 2·7 times the energy requirements for maintenance (458 kJ metabolisable energy/kg BW^0·75 per d^{( 26 )}). Feed refusals were collected 30 min after feeding.

Table 1 Composition of the experimental diets (as-fed basis)

NE, net energy; AID, apparent ileal digestible.

* Two levels of dietary protein supply (adequate or restricted (70 % of adequate)) were used in the study, at a similar daily supply of other nutrients. In the restricted dietary protein supply, the proportion of protein-containing ingredients in the diet was reduced by 30 % relative to the proportion in the adequate-protein diet. In order to supply all pigs with the same amount of the basal mixture, relative to their metabolic body weight, the feed allowance of pigs fed the restricted-protein diet was 94·3 % of those fed the adequate-protein diet.

† Vitamin and mineral premix provided per kg of adequate or restricted diet, respectively: 2·4 or 2·5 mg vitamin A; 50 or 52·5 μg cholecalciferol; 14·7 or 15·7 mg vitamin E; 1·5 or 1·6 mg vitamin K; 1·0 or 1·1 mg thiamin; 4·0 or 4·2 mg riboflavin; 12·0 or 12·6 mg pantothenic acid; 20·0 or 21·0 mg niacin; 20·0 or 21·0 μg vitamin B₁₂; 0·20 or 0·21 mg folate; 1·0 or 1·1 mg vitamin B₆; 100 or 105 mg choline chloride; 100 or 105 mg Fe as FeSO₄; 10·0 or 10·5 mg Cu as CuSO4.5H₂O; 65·0 or 68·3 mg Zn as ZnO; 30·0 or 31·5 mg Mn as MnO; 0·15 or 0·16 mg Co as CoSO₄; 0·75 or 0·79 mg K as KI; 0·30 or 0·31 mg Se as sodium selenite.

‡ Protastar^®, AVEBE Feed.

§ Unless indicated otherwise.

∥ NE was calculated based on Centraal Veevoederbureau^{( 59 )}.

At day − 16 or − 14 before the start of immune system activation, the pigs were surgically fitted with a jugular vein and a carotid artery catheter for blood collection and injection of a mixture of U-¹³C-labelled AA, respectively. Neopen (Neomycin 5 mg/kg BW and Procaïne benzylpenicillin 10 000 IU/kg BW; Intervet) was given intramuscularly 1 d before surgery, at surgery and 1 d after surgery. Flunixin (Finadyne 2·2 mg/kg BW; Schering-Plough) was given intramuscularly at surgery and for 2 d after surgery. A timeline of the experiment is shown in Fig. 1, with day 0 being the start of immune system activation by the i.v. administration of CFA (F5881; Sigma-Aldrich). CFA is a mineral oil containing 1 mg of dead Mycobacterium tuberculosis cells per ml. The dose of CFA administered per pig was 0·2 ml/kg BW, diluted with saline in a ratio of 1:2. The dose was spread over four equal sub-doses, of which two were infused at day 0 and two at day 1, in the morning between 09.15 and 10.30 hours, and in the afternoon between 15.15 and 16.30 hours. Of the pigs, eight did not receive the fourth sub-dose of CFA, as clinical observations after the first infusions on eight pigs showed a more severe response, i.e. greater and persistent feed refusals, and greater increase in respiratory rhythm, than expected based on a preliminary study (E Kampman-van de Hoek, unpublished results).

Fig. 1 Timeline of the experimental period. A, autopsy; BS, blood sampling; ILR, irreversible loss rate measurement by the injection of the U-¹³C-labelled amino acid mixture; i.v., intravenous; CFA, complete Freund's adjuvant.

Immunological response parameters

At days − 5, − 3, − 1, 3, 4, 5, 6, 7 and 8, blood samples were collected into serum tubes (Vacuette; Greiner Bio-One) and allowed to clot for 1 h at room temperature. Serum was collected after centrifugation for 10 min at 1800  g and was stored at − 20°C until analyses of albumin (Randox Bromocresol Green assay, catalogue no. AB 362), C-reactive protein (CRP, ELISA; Reactivlab Limited), haptoglobin (Tridelta Phase Haptoglobin Assay, catalogue no. TP-801), pig major APP (pigMAP, ELISA; Reactivlab Limited), and total protein (biuret reaction⁽ Reference Doumas, Bayse and Carter ^{27 )}). At days − 5, 0, 1, 3, 5 and 8, blood samples were collected into EDTA tubes (Vacuette; Greiner Bio-One) and analysed for the number of total leucocytes. At day 9, all pigs were euthanised and autopsy was performed by an experienced pathologist. Autopsy observations included assessment of body condition, visual inspection for abnormalities of the lungs, spleen, stomach, small intestine, large intestine, kidneys, liver, heart, and mesenteric lymph nodes, determination of lung weight, and histological evaluation of the lungs, liver, tracheobronchial lymph nodes and kidneys.

Nitrogen balance

Pigs were equipped with a Velcro support system to allow separate collection of the faeces⁽ Reference Van Kleef, Deuring and van Leeuwen ^{28 )} and urine. Faeces and urine were collected quantitatively from each pig during two periods of five subsequent days each, i.e. in the pre- and post-challenge periods (Fig. 1). Faeces were stored at − 20°C until analysis. Urine was collected via funnels, which were sprayed with an acetic acid buffer (sodium acetate 0·08 m, formic acid 0·025 m and acetic acid 0·013 m) to prevent evaporation of NH₃, into buckets containing sulphuric acid (4·5 m), to maintain a pH < 3 for conservation. Urine was collected daily from the buckets, weighed, sampled and stored at − 20°C until analysis. N content in the urine and fresh faeces was analysed using the Kjeldahl method^{( 29 )}. DM content of the faeces was determined by drying at 103°C^{( 30 )}.

Amino acid metabolism

At pre-challenge (day − 5), early post-challenge (day 3) and late post-challenge (day 8), the fluxes of plasma lysine, tryptophan, methionine, isoleucine, leucine, valine, phenylalanine and tyrosine (Lys, Trp, Met, Ile, Leu, Val, Phe and Tyr, respectively) were studied by measuring the change in plasma isotopic enrichment of individual AA in time after an intravenously administered bolus of these U-¹³C-labelled AA. To create a steady state in dietary AA supply at the day of injection of the U-¹³C-labelled AA mixture and frequent blood sampling, daily feed allowance was spread over ten equal meals. Of these, two meals were fed at 07.30 hours, followed by hourly meals from 09.10 hours until 16.10 hours. At 12.30 hours, a mixture of eleven U-¹³C-labelled AA (97–99 atom percent ¹³C; Cambridge Isotope Laboratories) was injected. The composition of the mixture (mg/g saline) was as follows: l-Lys, 0·17; l-Thr, 0·18; l-Trp, 0·07; l-Met, 0·06; l-Cys, 0·04; l-Ile, 0·16; l-Leu, 0·16; l-Val, 0·19; l-Phe, 0·13; l-Tyr, 0·16; l-histidine, 0·08. The mixture was injected as a bolus (0·50 g/kg BW; 0·25 ml/s) in the carotid artery. If the carotid artery catheter was blocked, the mixture was injected in the jugular vein. Blood samples (4 ml each) were collected from the jugular vein and transferred into tubes containing lithium heparin (Vacuette; Greiner Bio-One) at 10 min before the injection of the U-¹³C-labelled AA mixture and at 3, 5, 7, 9, 11, 15, 25, 45, 80 and 120 min after injection. The tubes were immediately placed on ice and centrifuged for 10 min at 2000  g at 4°C, after which plasma was collected and stored at − 20°C until analysis. In each blood sample, ¹³C enrichment was measured in plasma Lys, Trp, Met, Ile, Leu, Val, Phe and Tyr as ethyl chloroformate ester (ECF; Merck Schuchardt OHG) derivatives by GC–combustion–isotope ratio MS (Isotope Ratio MS, Delta V Advantage, Thermo Scientific; GC Trace Ultra, Thermo Scientific (column no. CP8982, VF-17ms 30 m × 0·25 mm, film 0·25 μm; Agilent Technologies); and combustion, Combustion III, Thermo Scientific), as adapted from Huang et al. ⁽ Reference Huang, Hogewind-Schoonenboom and de Groof ^{31 )}. Briefly, 20 μl hydrogen chloride (1 m) and 200 μl Dowex ion exchange resin (AG 50W-X8 H⁺ form, 200–400 mesh; Dow Chemical Company) were added to 180 μl plasma and eluted with 0·7 ml ammonium hydroxide (6 m) to isolate free plasma AA. The supernatant was evaporated with a centrifugal concentrator (Jouan RC 1022; Thermo Scientific) under vacuum at room temperature. Derivatisation was performed by adding 140 μl ethanol–pyridine (4:1, v/v) and 20 μl ECF to the dry supernatant. Derivates were extracted by adding 4 ×  200 μl hexane–dichloromethane–ECF (50:50:1, by vol.), and the supernatant was dried in a vial under N₂ gas at room temperature. After dissolving in 50 μl ethyl acetate, the sample was injected in triplicate into the GC. The ¹³C enrichment of histidine could not be successfully analysed due to high losses of histidine during the derivatisation step. The ¹³C enrichment of Thr and Cys could not be determined with the current procedure, and additional derivatisation steps would be required for their measurement.

Calculations

Dietary N intake, faecal and urinary N excretion and whole-body N retention were expressed relative to metabolic BW (kg BW^0·75). Relative lung weight was calculated as a percentage of BW. ¹³C enrichment in plasma AA was expressed as the tracer:tracee ratio (TTR). To calculate a change in the TTR in time, for each AA, the background enrichment (obtained from plasma samples taken before the injection of the U-¹³C-labelled AA mixture) was subtracted from ¹³C enrichment in samples after injection.

The ILR of AA from plasma was calculated from the change in the ¹³C enrichment of plasma AA after the intravenously administered bolus of U-¹³C-labelled AA using the model and calculations as described by Holtrop et al. ⁽ Reference Holtrop, Lapierre and Lobley ^{32 )}. The following assumptions were made: there is a physiological steady state during the measurement, i.e. a constant size of the plasma AA pool, so that the inflow of AA into the plasma pool equals the outflow from the plasma pool⁽ Reference Waterlow ^{14 )}; the tracer transfers along with the tracee between compartments with a constant fractional rate⁽ Reference Waterlow ^{14 )}; the ILR for an AA occurs as an output from the plasma pool, and only by the incorporation of the AA into synthesised protein or by the loss of the AA via oxidation⁽ Reference Reeds, Cadenhead and Fuller ^{33 )}. Finally, once the tracer has entered the body protein pool, there is no recycling of the tracer into the plasma pool, as the whole-body protein pool is a large pool with a low turnover rate compared with the plasma pool⁽ Reference Waterlow ^{14 )}. A double exponential model was fitted to the ¹³C enrichment of individual plasma AA after the administration of the bolus injection:

(1) $$ E ( t ) = a _{1}\,exp( b _{1} t ) + a _{2}\,exp( b _{2} t ), $$

where E(t) is the predicted ¹³C enrichment in plasma AA (TTR) at time t (min); and a ₁, b ₁, a ₂ and b ₂ are parameter estimates from which the ILR (μmol/kg BW per h) was calculated:

(2) $$ILR = d /( a _{1}/ b _{1} + a _{2}/ b _{2})60, $$

where d is the dose of the administered U-¹³C-labelled AA (μmol/kg BW).

For each AA and pig, the pool size, i.e. the amount of AA in the pool (μmol/kg BW), was calculated as:

(3) $$Pool size = d 0/( a _{1} + a _{2}). $$

An ILR index was calculated for each pig and time point as the ILR at day − 5, 3 or 8 divided by the mean ILR at days − 5, 3 and 8 of that particular pig, multiplied by 100. This index indicates the change in the ILR within animals as affected by the challenge.

AA released from protein breakdown was calculated as the difference between the ILR and dietary intake, using the steady-state model of Waterlow⁽ Reference Waterlow ^{14 )}, i.e. ILR = protein breakdown+dietary intake = protein synthesis+AA oxidation. Intake was estimated by multiplying the feed intake by the dietary apparent ileal digestible content of each AA and divided by 24 h and the molar mass.

The following two indices were calculated from serum concentrations of APP: a nutritional acute-phase index (NAPI), and a health status acute-phase index (HAPI). The NAPI was considered to be associated with the nutritional costs of APP synthesis, implying that the half-lives of the APP should be taken into account. The half-life of a positive APP was considered to be inversely related to the requirements for AA for APP synthesis. To amplify the nutritional costs of an APP response, all the measured positive APP are divided by the half-life (CRP 19 h⁽ Reference Vigushin, Pepys and Hawkins ^{34 )}, haptoglobin 132 h⁽ Reference Dobryszycka, Osada and Woźniak ^{35 )} and pigMAP 132 h, with the latter value being assumed to be similar to that of haptoglobin, based on the response pattern⁽ Reference Petersen, Nielsen and Heegaard ^{36 )}):

(4) $$NAPI = (pigMAP\ (g/l)/half\hyphen life) + (CRP\ (g/l)/half\hyphen life) + (haptoglobin\ (g/l)/half\hyphen life). $$

The HAPI was calculated as the sum of positive APP indices divided by the index for albumin as a negative APP, in which each index reflects the change in APP within a pig relative to the mean APP at days − 5, 3 and 8 of that pig. The HAPI was considered as a general indicator of health status. By including the indices for positive and negative APP in the HAPI, the range in values is amplified⁽ Reference Toussaint, Ederen and Gruys ^{37 ,} Reference Gruys, Toussaint and Niewold ^{38 )}:

(5) $$HAPI = \frac {CRP\ index + haptoglobin\ index + pigMAP\ index}{albumin\ index}, $$

where the APP index (e.g. CRP index) was calculated for each pig and time point as the APP concentration at days − 5, 3 or 8 divided by the mean APP concentration at days − 5, 3 and 8 of that particular pig, multiplied by 100.

Statistical analysis

Pig was considered as the experimental unit. The effects of dietary treatment and collection day or period on leucocytes, N balance measures, ILR, AA release in plasma from protein breakdown, and AA plasma pool size were analysed with a mixed model, with collection day, or period, taken as the repeated measure. Fixed effects also included the interaction between dietary treatment and collection day, or period. The effects were analysed by pairwise comparisons using Tukey–Kramer adjustment. A covariance structure was chosen based on the lowest value for the Akaike and Bayesian information criteria. The effects of dietary treatment, collection day and the interaction between the two on APP and total protein serum concentrations were analysed separately per period (pre- and post-challenge) with a mixed model, with collection day taken as the repeated measure. For the post-challenge APP serum concentrations, the mean of pre-challenge serum APP concentrations (days − 5, − 3 and − 1) was used as a covariate. The effect of dietary treatment on relative lung weight was analysed by ANOVA. To associate a change in AA utilisation with a change in APP concentrations or N balance, the correlation between the ILR index for AA and the NAPI or HAPI, and the correlation between N retention and the ILR or ILR index were determined using a Pearson correlation analysis. To distinguish between the 2 d post-challenge (days 3 and 8), the correlation analyses were performed separately in two parts, i.e. including data of pre-challenge and day 3 post-challenge, and including data of pre-challenge and day 8 post-challenge.

The normality of the distribution of studentised residuals was assessed. Data on pigMAP and CRP were log transformed to obtain the normal distribution of model residuals. All statistical procedures were conducted in SAS (SAS Institute, Inc.). Data are presented as means with their pooled standard errors, and the effects were considered significant at P≤ 0·05.

The goodness-of-fit of the double exponential model used to fit the ¹³C enrichment of individual plasma AA was assessed by the mean square prediction error (MSPE). The root MSPE was scaled to the observed mean (mean prediction error), and the correlation between the predicted and observed values was calculated. Errors due to overall bias, due to the deviation of the regression slope from unity, and due to random variation were calculated⁽ Reference Bibby and Toutenburg ^{39 )}. Enrichment data of some AA were excluded due to unrealistic parameter estimation and concomitant unrealistic ILR.