Animals and experimental design

The experiment was conducted as a block experiment with four dietary treatments and the same sixteen pigs were measured four times from weaning until 80 kg. Two blocks (A and B) were used and the blocks were measured with one-week in-between. In each block eight recently weaned barrows [(Landrace × Yorkshire) × (Hampshire × Duroc)] from two litters were used. One pig from each litter was allocated to one of the four dietary treatments. At arrival the barrows in block A weighed 8.2 ± 0.6 kg (mean ± s.d.) and the barrows in block B 9.8 ± 0.9 kg. Four spare pigs having the same age as the barrows in block A were fed the control diet.

The experimental diets were fed from day one after arrival. At 9 days after arrival the pigs were placed in metabolism cages and the first 4-day balance period started at 12 days after arrival. Another three balance periods were conducted at 40, 68 and 96 days after arrival. Once during each balance period the barrows were subjected to a 22-h respiration experiment by means of indirect calorimetry in an open-air circulation system (Chwalibog et al., Reference Chwalibog, Tauson and Thorbek2004).

Diets

The batch of BPM (Bioprotein®, Norferm AS, Stavanger, Norway) used in this experiment was pelleted with inclusion of approximately 1% soya oil after spray-drying in order to minimise dusting. All ingredients were then mixed and the diets pelleted. In order to use diets that were in agreement with the actual nutritional requirement of the pigs, diets designed for weaned piglets were used in periods 1 and 2, and diets designed for growing-finishing pigs were used in periods 3 and 4. The BPM content of the starter and growing finishing diets remained the same, but the N and energy contents were somewhat reduced in the growing-finishing diet in order to comply with the animals' decreasing protein requirements. The starter diet was used from arrival until the end of balance period 2, and the growing-finishing diet was used during the rest of the experiment. One of the experimental diets served as the control diet and contained no BPM (BP0), while the remaining diets contained 5% BPM (BP5), 10% BPM (BP10) and 15% BPM (BP15) (Table 1). The BPM replaced SBM on a digestible protein basis, providing 0/0, 17/17, 33/35 and 49/52% of N in the starter and growing-finishing diets, respectively. The contents of digestible protein were calculated by using digestibility values indicated by Skrede et al. (Reference Skrede, Berge, Storebakken, Herstad, Aarstad and Sundstøl1998) for BPM, and table values for the other feed ingredients (Norwegian Feed Table, 2002). The diets were formulated to meet or exceed the requirements for essential amino acids and all other nutrients established by the National Research Council (NRC, 1998). The diets were produced by the Centre for Feed Technology (Ås, Norway) and pelleted using a 3-mm die on a Münch pellet press (Münch-Edelstahl GmbH, Hilden, Germany). For a more detailed description of the diet formulation, see Øverland et al. (Reference Øverland, Kjos and Skrede2004). All diets were analysed for DM, ash, N, fat, energy, amino acids, purine and pyrimidine bases (Table 1).

Table 1 Composition and chemical content of the diets used in balance and respiration experiments with pigs

^†Vitamins and trace elements included to provide the following per kg of feed: 140 mg Zn; 201 mg Fe; 80 mg Mn; 20 mg Cu; 10 mg I, 0.4 mg Se; 3 300 μg retinol; 34.4 μg cholecalciferol; 137.5 mg d-α-tocopheryl acetate; 6.9 mg riboflavin; 22.9 mg d-pantothenic acid; 27.5 μg cyanocobalamin.

^‡Vitamins and trace elements included to provide the following amounts per kg of feed: 105 mg Zn; 75 mg Fe; 60 mg Mn; 15 mg Cu; 7.44 mg I; 0.3 mg Se; 2 520 μg retinol, 17.5 μg cholecalciferol; 115.9 mg d-α-tocopheryl acetate; 5 mg riboflavin; 15 mg d-panthothenic acid; 20 mg cyanocobalamin.

Housing and feeding

The pigs were housed individually for the duration of the experiment. For the first 9 days after arrival and between balance periods they were housed in pens with concrete floors covered with wood shavings. During the balance periods the pigs were housed in metabolic cages of stainless steel, (1.65 m × 0.75 m with a slatted floor of round stainless steel bars). When kept in the balance cages and the pens, but not in the respiration chambers, the pigs had visual contact. The light schedule was 12 h light and 12 h dark. Between balance periods the pigs were fed twice daily (0830 and 1530 h) but during balance periods they were fed once daily between 1130 and 1200 h. The feed supply was regulated on a daily basis to a level where pigs had a minimum of feed residues, i.e. were fed as close to ad libitum as possible. Between balance periods, water was provided ad libitum from drinking nipples. During the balance periods, water (twice the weight of the feed) was mixed into the diets. In addition, pigs were given drinking water in a trough. The temperature was kept at 20 to 22 °C throughout the experimental period. All pigs were provided with a rubber mat in the front of the metabolism cages during the first and second balance periods.

Experimental techniques

Pigs were weighed at the start and end of each 4-days balance period. The collection procedures were performed between 0800 and 1200 h every day. Feed residues, faeces and urine were quantitatively collected from the individual pigs, weighed and frozen at − 18°C. Urine was collected in 30 ml of 5% sulphuric acid in periods 1 and 2 and in 50 ml of 5% sulphuric acid in periods 3 and 4. For 2 days in periods 2 and 4 when protein turn-over was estimated by means of the ¹⁵N-glycine end-point technique the addition of acid was omitted. The results from the protein turn-over experiment will be reported elsewhere (Hellwing et al., Reference Hellwing, Tauson, Skrede, Kjos and Ahlstrøm2007).

The inside surfaces of the metabolic cage, the mat and collection plate were washed with citric acid daily after completion of the collection procedures. After each balance period feed residues, faeces and urine were thawed and mixed to homogeneity. Samples for chemical analyses were taken and frozen at − 18°C for later analyses. Furthermore, samples of faeces were freeze-dried for analyses of ash, fat and energy. The citric acid rinse was thawed and centrifuged at 3000 × g for 10 min to separate the solid particles (assumed to be faeces residues) from the fluid (assumed mainly to contain N residues derived from urine). The sediment was weighed and freeze-dried. A sample of the supernatant was stored at − 18°C.

The day when the pigs were subjected to the respiration experiment they were brought to the respiration unit between 0930 and 1030 h. Each respiration experiment lasted 22 h, starting at 1100 h and ending at 0900 h the following morning. The volume of each respiration chamber was 3500 l and the chambers were constructed for animals with live weights of 5 to 200 kg. For a detailed description of the calibration and measurement procedures, see Chwalibog et al. (Reference Chwalibog, Tauson and Thorbek2004).

Analyses

Samples of diets and freeze-dried faeces were ground and homogenised before analyses. Feed residues were analysed for DM, assuming that the composition of the DM was the same as in the DM of the feed. Wet faeces were analysed for DM and N and freeze-dried faeces for ash, fat and energy. Urine was analysed for N. The supernatant of the citric acid rinse was analysed for N, and the DM content of the sediment was determined by freeze-drying.

DM was determined by evaporation at 105°C to constant weight. Ash was determined by incineration at 525°C. N was determined by the micro-Kjeldahl technique using the Tecator–Kjeltec system 1030 (Tecator AB, Höganäs, Sweden). CP was calculated as N × 6.25. Fat was determined by petroleum ether extraction in a Soxtec system after HCl hydrolysis. Gross energy was determined using an adiabatic bomb calorimeter (IKA Calorimeter system, IKA Gmbh and Co. KG, Staufen, Germany). The amino acids, except tryptophan, in the diets were determined according to the European Community (1998). Tryptophan was analysed according to the Bech-Andersen (Reference Bech-Andersen1991) procedure. Adenine, guanine, thymine, uracil, and cytosine in the diets were determined by a HPLC method. A diet sample of 0.100 g was mixed with 2 ml of HClO₄ and heated for 1 h at 95°C. The sample was chilled and mixed with 5 ml borate buffer and 3 ml 12.4 mmol/l KOH. A sample of 1 ml was taken and centrifuged at 15 000 r.p.m. for 10 min. To the centrifuged sample 4 ml borate buffer was added and micro-filtrated (0.45 μm). The sample was injected into the column and eluents were detected by UV-absorbance at 254 nm. Data were analysed against external standards using the Hewlett-Packard HP ChemStation Software (Møller-Hansen, personal communication).

Calculations

Urinary nitrogen (UN) was calculated as the sum of the N in the urine and the citric acid rinse. Faecal nitrogen (FN) was calculated as the N content of the faeces plus the N content of the sediment from citric acid rinse. It was assumed that the N content of the sediment was the same as that of the faeces. Energy in urine (UE) was calculated as 53.5 kJ/g × UN (Chwalibog et al., Reference Chwalibog, Tauson and Thorbek2004). RN was calculated as ingested nitrogen (IN) minus UN and FN. Metabolisable energy (ME) was calculated by subtracting FE and UE from gross energy intake. Heat production (HE) was calculated according to Brouwer (Reference Brouwer and Blaxter1965) as HE, kJ = 16.18 × O₂, L+5.02 × CO₂, L − 5.99 × UN, g − 2.17 × CH₄, L. The production of CH₄ was low and therefore omitted from the equation. Retained energy (RE) was calculated as ME minus HE. The non-protein respiratory quotient (RQ_np) was calculated as RQ_np = (CO₂, L–[UN, g × 6.25 × 0.774])/(O₂, L–[UN, g × 6.25 × 0.957]). Furthermore, the maximum protein retention was calculated according to a second order equation as described, and under the same assumptions, as given by Chwalibog et al. (Reference Chwalibog, Jakobsen and Thorbek1996) and Tauson et al. (Reference Tauson, Chwalibog, Jakobsen and Thorbek1998).

Statistical analyses

Statistical analyses of data from the balance and respiration experiments were carried out by means of the MIXED Procedure in Statistical Analysis Systems Institute (SAS) (Littell et al., Reference Littell, Milliken, Stroup and Wolfinger1996) using the following model:

where Y _ijkl is the Y _ijklth observation, μ is the general mean, α_i is the fixed effect of diet (BP0, BP5, BP10 and BP15), β_j is the fixed effect of balance period (1 to 4), αβ _ij is the interaction between diet and balance period, γ_k is the fixed effect of block (A and B) and ɛ_ijkl is the residual error. Data were analysed as repeated measurements and the heterogeneous autoregressive order 1 (ARH(1)) covariance structure was fitted (Littell et al., Reference Littell, Milliken, Stroup and Wolfinger1996). Results are presented as least squares means (LSmeans) and the square root of residuals (RR) is given for each variable. Pair-wise comparisons of LSmeans were made using the PDIFF option, and effects were considered significant if P < 0.05. One observation from period 2 was omitted because of an injury not related to the dietary treatment. Another three observations (regarding one pig in period 2 and two pigs in period 3) were omitted from the analysis of the respiration data because of technical problems. A linear regression analysis of the percent of N derived from BPM and apparent digestibility of N was performed using PROC REG in SAS (1990).