Diets

Four isoenergetic and isofibrous diets were formulated to induce differences in the ileal flow of crude protein (CP) through changes in the dietary level and the apparent ileal digestibility of protein. A basal diet with a high protein and lucerne hay content (HPHL) was formulated according to De Blas and Mateos (Reference De Blas, Mateos, de Blas and Wiseman1998) and recent works on optimal starter feed composition (Gutiérrez et al., Reference Gutiérrez, Espinosa, García, Carabaño and De Blas2002a and Reference Gutiérrez, Espinosa, García, Carabaño and De Blasb and Reference Gutiérrez, Espinosa, García, Carabaño and De Blas2003). Another diet (LPHL; low CP, high lucerne hay) was designed by substituting dietary starch for CP, maintaining the apparent ileal CP digestibility of the diets according to an estimation made from previous works (García et al., Reference García, De Blas and Carabaño2005). Two additional low protein diets were formulated further to reduce the ileal flow of protein by replacing lucerne hay in diet LPHL with a more digestible protein source (soya-bean protein concentrate) plus a mixture of fibrous ingredients (sunflower hull, sugar beet and apple pulp), totally (LPLL) or partially (LPML). All the diets were pelleted and included 5 g/kg of lucerne hay marked with an indigestible marker (ytterbium) according to the procedure described by García et al. (Reference García, Carabaño and De Blas1999). The ingredients and chemical composition of the diets are shown in Tables 1 and 2.

Table 1 Ingredients in the experimental diets (g/kg)

† HPHL =  high protein high lucerne-hay. LPHL =  low protein high lucerne-hay. LPML =  low protein medium lucerne-hay. LPLL =  low protein low lucerne-hay.

‡ Provided by Trouw Nutrition España S.A. (Madrid, Spain): mineral and vitamin composition (mg/kg feed): Mg, 290; Na, 329; S, 275; Co, 0.7; Cu, 10; Fe, 76; Mn, 20; Zn, 59.2; I, 1.25; choline, 250; riboflavin, 2; niacin, 20; pyridoxine, 1; phytylmetaquinone, 1; alpha-tocopherol, 13; thiamine, 1; retinol, 2.5, and cholecalciferol, 0.019.

Table 2 Chemical composition of experimental diets (g/kg dry matter)

† HPHL =  high protein high lucerne-hay. LPHL =  low protein high lucerne-hay. LPML =  low protein medium lucerne-hay. LPLL =  low protein low lucerne-hay.

Faecal digestibility trial

Forty rabbits weighing 464 (s.e. 18) g at 25 days of age, were blocked by litter and assigned at random to the experimental diets (10 per diet) to determine the apparent faecal digestibility of dry matter (DM), CP and energy. Rabbits were individually caged and had ad libitum access to the food during the experimental period. Following a 1-week adaptation period, the feed intake and total faecal output (caecotrophy was not prevented) were recorded from 32 to 35 days of age. The faeces daily collected were stored at − 20°C, dried at 80°C for 48 h and ground to pass a 1-mm sieve for analysis.

Ileal digestibility trial

Sixty four rabbits weighing 454 (s.e. 19) g at 25 days of age were blocked by litter and assigned at random to the experimental diets (16 per diet) to determine the apparent ileal digestibility of DM, CP and amino acids (AA). Following a 10-day adaptation period, animals were slaughtered by cervical dislocation weighing 788 (s.e. 33) g. Slaughter time was between 1900 and 2100 h to avoid the influence of caecotrophy on the chemical composition of the digesta (Merino and Carabaño, Reference Merino and Carabaño2003). The last 20 cm of the ileum were taken and the ileal contents were removed, frozen and freeze-dried. The samples were then ground and, because of the small quantity available, they were pooled in groups of two rabbits of the same treatment to analyse CP and ytterbium. To determine the AA content of the ileal digesta, a fixed amount (0.05 g) of all the samples belonging to each treatment were pooled. Ytterbium content of experimental diets and ileal digesta were analysed to calculate apparent ileal digestibility of CP and AA (CP_id and AA_id according to the following equations):

Digestive traits trial

Sixty weanling mixed-sex rabbits (15 animals per diet) 25 days old and weighing 501 ± 16 g, were fed the experimental diets up to 35 days of age. Final weight was 922 ± 43 g. Rabbits were individually caged and had ad libitum access to the food during the experimental period. Animals were slaughtered by cervical dislocation between 1900 and 2100 h to avoid the caecotrophy period. After that, the gastro-intestinal tract was removed and weighed. Stomach and caecum were weighed separately with and without their contents. The pH of caecal and stomach contents was determined. In the stomach digesta, three measurements of pH were taken: at the pyloric and fundus areas, and in the mixture of both areas. A sample was taken from the middle part of the jejunum of each animal to determine mucosa histology. The samples were placed in a 10% buffered neutral formaldehyde solution (pH 7.2 to 7.4) and were gradually dehydrated with increasing concentrations of ethyl alcohol (50 to 100%). These dehydrated specimens were first embedded in paraffin, prepared by sectioning at 6 μm, and stained with hematoxylin and eosin. The sections were analysed under a light microscope (Olympus BX40, Olympus Optical Co., 20 097, Hamburg, Germany) to determine their morphometric index by computer-assisted image analysis (The ImageJ v 1.26. Wayne Rasband, National Institutes of Health, Bethesda, MD 20 892, USA). Villi heights (from the top of the villi to the villi crypt junction) at three cross sections were measured according to Hampson (Reference Hampson1986) from the mean value of 30 vertically oriented villi per animal.

Finishing performance trial

Two hundred and eight New Zealand White × California weanling mixed-sex rabbits (52 per diet), 25 days old and 494 ± 13 g live weight, were blocked by litter and assigned at random to the experimental diets. After weaning, rabbits were individually caged and were fed the experimental diets through a 2-week period. Drinking water was supplemented during this period with a mixture of 100 mg/kg of apramicine sulphate and 120 mg/kg of tylosin. After 39 days of age, all the animals received a commercial feed (CUNIUNIC®, NANTA, S.A.: 170 g CP, 144 g starch, 373 g neutral-detergent fibre (NDF) and 49 g acid-detergent fibre (ADF) per kg) until they reached 56 days of age. Animals had ad libitum access to the feed and water throughout the whole experimental period. Feed intake, weight gain and mortality rate at day 14 after weaning and at the end of the experimental period were recorded per cage. Mortality rate was also controlled in another group of 280 rabbits (70 per diet) weighing 498 ± 13 g at 25 days of age. Animals were blocked by litter and assigned at random to the same dietary treatments, but they were not supplemented with antibiotics.

Ileal microbiota characterisation trial

One hundred and twenty 25-day-old rabbits (30 per diet) weighing 448 ± 19 g live weight, were blocked by litter and assigned at random to the experimental diets during 10 days. Within each treatment, 18 animals received antibiotic supplementation in drinking water (100 mg/kg of apramicine sulphate and 120 mg/kg of tylosin), whereas the other 12 rabbits were not supplemented. At 35 days of age the rabbits, weighing 860 ± 30 g, were slaughtered by cervical dislocation between 1900 and 2100 h. One g of ileal digesta was collected in a sterile plastic tube that contained 3 ml of 98% molecular biology grade ethanol and were stored at 4°C to be analysed by RFLP according to the following procedure:

A 400-mg sample of gut contents was processed for total DNA extraction using the QIAamp DNA Stool Mini Kit (Qiagen Inc., Chatsworth, CA) system, in accordance with the instructions of the manufacturer with two additional steps of lysozyme and proteinase K. The purified DNA was maintained at − 20°C until use. Two primers (5′-CTACGGGAGGCAGCAGT-3′ and 5′-CCGTCWATTCMTTTGAGTTT-3′) for regions I and II of the 16S rRNA gene (Lane, Reference Lane, Stackebrandt and Goodfellow1991), were used to amplify a DNA segment of 500-600 bp. PCR mixtures (PCR-Master Mix – Applied Biosystems – with 1.25 IU of Taq polymerase, 50 ng of DNA template, 0.2 μmol/l the preceding primers, and distilled water in a total volume of 50 μl) were heated to 94°C for 5 min once, followed by 35 cycles of denaturation at 94°C for 1 min, primer annealing at 45°C for 1 min, and DNA extension at 72°C for 1 min 15 s. The last extension cycle was continued for 5 min. Aliquots of the amplified DNA fragments were digested, in separated tubes, with Alu I, Rsa I, Hpa II, Sau 3A I or Cfo I restriction endonucleases (Sigma-Aldrich) in accordance with manufacturer specifications. The endonuclease fragments were solved in 2% wide range agarose by electrophoresis at 150 V for 60 min. The bands of DNA were visualised in an UV Chemigenious Image System (SynGene) using the GeneSnap software (SynGene). Pictures with 4.63 s exposure were stored. With the information resulting from the relative size of the restriction fragment length polymorphism (RFLP) bands, the information stored in the ‘SSU_Una.gb’ file from the Ribosomal Database Project (Maidak et al., Reference Maidak, Olsen, Larsen, Overbeek, McCaughey and Woese1997), and a specific software developed in our Institute, we could identify the bacterial genus or species compatible with the obtained RFLP profile. From each animal a biodiversity degree, defined as the number of 16S r-DNA sequences, deposited in the Ribosomal Database Project, compatible with the RFLP profile obtained from the total DNA extracted from the gut samples, was recorder. Also, the frequency of the compatibility profile of every bacteria studied defined as the presence or absence of RFLP bands compatible with the theoretical RFLP bands for a certain genus or bacterial species was studied for every animal (i.e. a combination of bands with 92 bp+467 bp in AluI, plus 120 bp+404 bp+35 bp bands in RsaI, plus 189 bp+58 bp +312 bp bands in HpaII, plus 82 bp+477 bp bands in Sau3A, plus a band of 559 bp in CfoI is compatible with C. perfringens. The absence of any of the above mentioned bands in the RFLP profile infer that the level of C. perfringens in the sample is below the detection level, as in other PCR-electrophoresis methods around 10⁴-10⁵ DNA copies per g of sample).

Housing

Animals were housed in wire metabolism cages measuring 250 × 600 × 330 mm. A cycle of 12 h of light and 12 h of dark was used throughout the experiment. The light was switched on at 0730 h. Heating and forced ventilation systems allowed the building temperature to be maintained between 18 and 23°C throughout the experiment. Rabbits were handled according to the principles for the care of animals in experimentation published by the Spanish Royal Decree 1201/2005 (2005). Because the trials were carried in a farm affected by epizootic rabbit enteropathy (ERE), animals were supplemented with antibiotics (100 mg/kg of apramicine sulphate and 120 mg/kg of tylosin) in drinking water. Mortality and ileal microbiota characterisation trial were additionally developed without supplementation in drinking water.

Analytical methods

Chemical analysis of diets and faeces was performed using the procedures of Association of Official Analytical Chemists (2000) for DM (930.15), ash (923.03), Dumas N (968.06) and starch (according to the alpha-amyloglucosidase method, 996.11). NDF, ADF and acid-detergent lignin were determined according to the sequential method of Van Soest et al. (Reference Van Soest, Robertson and Lewis1991). Gross energy (GE) was measured by adiabatic calorimetry. AAs were determined following acid hydrolysis using a Beckman System 6300HPA amino acid analyser (Fullerton, CA, USA). Samples were hydrolysed by reflux in 25 ml of 6 mol/l HCl with 10 g/l added phenol for 24 h at 120 °C. For the determination of sulphur amino acids (methionine and cystine), samples were oxidised with performic acid at 0 °C for 16 h and then, neutralised with 0.5 g of sodium meta-bisulphite before analysis. Tryptophan, being destroyed during acid hydrolysis, was not determined. Ytterbium content of diets and ileal digesta were analysed by atomic absorption spectrometry (Smith Hieftje 22, Thermo Jarrel Ash, MA, USA) using predosed samples to prepare common matrix standards. Previously, samples were ashed (600°C) and then digested by boiling with a solution of 1.5 mol/l HNO₃ and KCl (3.81 g/l).

Statistical analysis

Data from ileal and faecal digestibility, digestive traits and growth trials were analysed as a completely randomised-block design using type of diet as main effect and litter as block effect, by using the GLM procedure of Statistical Analysis Systems Institute (1991). Treatment sums of squares were partitioned into the effect of dietary level of protein (contrast of diets HPHL v. LPHL) and the linear and quadratic effects of level of substitution of lucerne hay with soya-bean protein concentrate (diets LPHL, LPML and LPLL). Weaning weight was used as a linear covariate in the growth traits analyses.

To analyse mortality, biodiversity degree and frequency of the compatibility profile, type of diet, antibiotic supplementation and their interaction were used as main effects. Mean comparisons of mortality and frequency of the compatibility profile traits were made using a chi-square test. Regression procedures were used to relate fattening mortality with frequency of the compatible profile of several entero-pathogenic bacteria.