Animals and diets

The Swiss Cantonal Committee for Animal Care and Use approved all procedures involving animals.

The experiment included a total of 36 Swiss Large White EMs originating from 12 litters. From weaning until the start of the experimental period (mean±SE BW=50.4±1.11 kg; age=105±0.3 days), EMs were group-penned and had ad libitum access to a commercial starter (mean±SE BW=10.8±0.44 to 27.2±0.25 kg) and grower diet (mean±SE BW=27.2±0.25 to 50.4±1.11 kg). At the end of the starter period, the littermates were allocated to the three experimental diets according to BW. The three diets consisted of a negative control diet (C) with no added tannins and two diets containing per kg of diet 15 (T15) or 30 g (T30) of supplementary tannins, respectively (Table 1). All diets were formulated to be isonitrogenous and isocaloric and tannin supplement, which originated from chestnut (Silvateam, San Michele Mondovì, Italy), was interchanged by straw meal. The experimental diets were offered ad libitum in a pelleted form. The pigs were reared in the finisher period in group pens, equipped with an automatic feeder and individual pig recognition system (Schauer Maschinenfabrik GmbH & Co. KG, Prambachkirchen, Austria) as described previously by Bee et al. (Reference Bee, Jacot, Guex and Biolley2008), which allowed the determination of individual feed intake in group housed pigs.

Table 1 Feed ingredients (%), nutrient and tannin composition of the experimental diets

DM, dry matter; DE, digestible energy.

¹ Control=standard finisher diet without addition of chestnut tannin powder; T15=standard finisher diet with addition of 1.5% of chestnut tannin powder; T30=standard finisher diet with addition of 3% chestnut tannin powder.

² 50% fat from beef and 50% fat from swine.

³ Chestnut powder.

⁴ Binder that aids in pellet formation.

⁵ Supplied the following nutrients per kg of diet: 20 000 IU vitamin A, 200 IU vitamin D₃, 39 IU vitamin E, 2.9 mg riboflavin, 2.4 mg vitamin B₆, 0.010 mg vitamin B₁₂, 0.2 mg vitamin K₃, 10 mg pantothenic acid, 1.4 mg niacin, 0.48 mg folic acid, 199 g choline, 0.052 mg biotin, 52 mg Fe as FeSO₄, 0.16 mg I as Ca(IO)₃, 0.15 mg Se as Na₂Se, 5.5 mg Cu as CuSO₄, 81 mg Zn as ZnO₂, 15 mg Mn as MnO₂.

⁶ The DE coefficients from each feed ingredient were obtained from the Swiss (Agroscope, 2015) database, respectively. Taking into account the relative amount of each feed ingredient in the diet, DE content was calculated.

Slaughter procedure and carcass measurements

One week after pigs reached 100 kg BW, they were selected for slaughter. Feed was withdrawn 16 h before slaughter by negating access to the feeder for the selected pigs. Avoiding all unnecessary stress, the EMs were walked ~100 m to the stunning area, and allowed to rest for 10 min before they were subjected to CO₂ stunning for 100 s, after which they were exsanguinated, scalded, mechanically dehaired and eviscerated. At this point the internal organs were removed, and the liver, kidney, testicles, salivary (mandibular) and bulbourethral glands were weighed. Within 2 min after evisceration, liver excisions were rinsed with a phosphate-buffered saline solution and stored at −20°C in RNA-Later solution (1018087; Qiagen, Basel, Switzerland) until RNA extraction. The hot carcasses were then weighed and the pH and temperature of the longissimus dorsi muscle (LD) was measured at the 10^th rib location before being refrigerated at 3°C for 1 day. One day postmortem, the left cold carcass sides were weighed and dissected into the major primal cuts (shoulder, loin, ham and belly) and trimmed free of all external fat as previously described (Bee et al., Reference Bee, Chevillon and Bonneau2004).

Feed analysis

Feed samples were milled using a 1.0-mm sieve (Brabender, Duisburg, Germany) before analysis. Dry matter content was determined after samples were dried at 105°C for 3 h and ash content was subsequently determined after incineration at 550°C. Nitrogen was determined using Kjeldahl procedure (Leco FP-2000 analyser; Leco, Mönchengladbach, Germany) and CP calculated by 6.25×N. Crude fibre was analysed after digestion with successively H₂SO₄ and KOH, washed with acetone, dried at 130°C and finally ashed (EN 71/393, ISO 6865:2000, VDLUFA 6.1.4). Crude fat of diets was determined as petrol ether extract after an acidic hydrolysis (ISO 6492:1999, VDLUFA 5.1.1).

The content of gallic acid and HT in the diets were determined as recently described by Johnson et al. (Reference Johnson, Ives, Ahern and Salminen2014). In brief, phenolic composition of the chestnut tannin extract and the four diet samples were quantified using 20 mg of finely ground powder extracted in 2×1.4 ml of acetone : water (8 : 2, v/v) for 3 h with a Vortex-Genie 2T mixer (Scientific Industries, Bohemia, NY, USA). After 10 min of centrifugation at 16 000×g (Eppendorf centrifuge 5402; Eppendorf AG, Hamburg, Germany), supernatant was stored in a separate vial and the extraction was repeated on the original tissue with fresh solvent. Acetone was removed from the pooled extracts using an Eppendorf concentrator 5301 (Eppendorf AG) and the sample was freeze-dried. Before analysis, sample was dissolved in 2 ml of water and filtered through a 0.20-µm polytetrafluoroethylene filter. Phenolics were analysed from each sample using ultra performance liquid chromatography with diode array and electrospray MS detectors (UPLC-DAD-MS, Waters Acquity UPLC and Waters Xevo TQ triple quadrupole mass spectrometer; Waters Corporation, Milford, MA, USA). We used a Waters Acquity UPLC BEH Phenyl (1.7 ml, 2.1 9100 mm) column with CH₃CN (A) and 0.1% HCOOH as eluents (Engström et al., Reference Engström, Pälijärvi and Salminen2015). Individual HTs were identified on the basis of their UV and MS spectra (Moilanen et al., Reference Moilanen, Sinkkonen and Salminen2013). Gallic acid was quantified in gallic acid equivalents, all gallic acid derivatives in pentagalloylglucose equivalents and ellagitannins as tellimagrandin I equivalents.

Analysis of indole, skatole and androstenone concentrations in the adipose tissue

Androstenone, skatole and indole concentrations in the adipose tissue were analysed according to Ampuero Kragten et al. (Reference Ampuero Kragten, Verkuylen, Dahlmans, Hortos, Garcia-Regueiro, Dahl, Andresen, Feitsma, Mathur and Harlizius2011) and based on the method previously described by Hansen-Møller (Reference Hansen-Møller1994). In brief, the adipose tissue samples were liquefied in a microwave oven for 2×2 min at 250 W. The liquefied lipids were centrifuged for 2 min at room temperature. The water was then removed and 0.5 ml of water-free liquid fat, kept at around 47°C, was placed in 2.5-ml Eppendorf tubes in duplicates and an internal standard was added (1 ml methanol containing 0.496 mg/l androstanone and 0.050 mg/l 2-methylindole). After vortexing for 30 s, the tubes were incubated for 5 min at 30°C in an ultrasonic water bath, kept at 0°C in ice-water bath for 20 min and then centrifuged at 11 000×g for 20 min. Finally, the liquid fraction was filtered (0.2-μm filter) and transferred into a vial for androstenone, skatole and indole analysis with an HPLC system. Concentrations were expressed per gram of adipose tissue. The quantification limits were 0.3 μg/g adipose tissue for androstenone and 0.03 μg/g adipose tissue for skatole and indole.

RNA isolation

Total RNA was extracted using a Nucleospin RNA XS kit (740902; Macherey-Nagel, Oensingen, Switzerland) following the procedure provided by the manufacturer. In brief, after thawing, 3 to 4 mg of liver tissue was homogenised in a MiniLys Bertin (Labgene, Chatel-St-Denis, Switzerland) using CK14 Precellys Lysing Kit (KT03961-1-203; Labgene) in 0.3 ml of RA1 buffer of the Nucleospin RNA XS kit. The RNA concentration was determined using a NanoDrop ND 1000 spectrophotometer (Witec AG, Littau, Switzerland). The mean 260/280 absorbance ratio of the samples was 2.13.

Primer design, reverse transcription and quantitative real-time PCR

For reverse transcription with the Quantitect Reverse Transcription kit (205311; Qiagen, Basel, Switzerland), which also includes a DNase I digestion step, 250 ng of RNA were used. The resulting reaction product was diluted 1 : 1 with RNAse-free water before further analysis. Primers for cytochrome P450 (CYP) isoenzyme CYP1A2 and CYP2E1 and CYP2A19 were designed using Primer-Blast service (Ye et al., 2012) offered by the National Institute of Health and verified for specificity using National Center for Biotechnology Information database (www.ncbi.nlm.nih.gov). Primers for the CYP1A2 gene were the same as used by Rasmussen et al. (2011). The target and housekeeping gene primers and National Center for Biotechnology Information accession numbers are shown in Supplementary Table S1. For each primers pairs, the efficiency of amplification was determined in three independent experiments.

Genes encoding CYP1A2, CYP2E1 and CYP2A19 were evaluated for their expression in pig livers via quantitative real-time PCR, using a KAPA Sybr Fast qPCR Kit (KK 4602m; Kapa Biosystems, Labgene, Chatel-St-Denis, Switzerland) with an Eco Illumina-Real Time PCR System (Labgene). The programme consisted of a pre-incubation step at 95°C for 5 min, followed by 40 cycles of 5 s at 95°C and 20 s at 62°C. The expression of each targeted gene was evaluated using $$\Delta \Delta ^{{{\minus}C_{t} }} $$ method (with efficiency corrections) and normalised using glyceraldehyde-3-phosphate dehydrogenase (GAPDH) as housekeeping genes. All the calculations were performed using Eco-Illumina Study software (Labgene).

Sensory analysis

The sensory test aimed to determine differences in intensity of boar taint odour and flavour as well as additional sensorial characteristics of cooked loin chops related to the dietary HT supply. The panel, which consisted of eight judges (five females and three males, from 35 to 62 years of age), was previously trained to determine boar taint as well as juiciness and tenderness. In addition, by using LD samples collected from the experimental animals, judges completed four-training sessions in order to agree on the following three discriminant descriptors: ‘bitter’, ‘gummy’ and ‘astringent’. For the traits juiciness, tenderness, bitter, gummy and astringent a monadic linear scale ranging from 0 to 10 (0=low intensity, weak; 10=great intensity, strong) was used. By contrast, for the boar taint assessment the judges indicated the presence or absence of boar taint odour and flavour using R-index technique (O’Mahony, 1988). The judges could give one of the four following answers regarding boar taint odour and flavour in the test as compared with the control sample: S (the flavour and odour was definitely present), S? (flavour and odour was present but they were not sure), N? (flavour and odour was not present but they were not sure) or N (flavour and odour was not present and they were sure). Samples were offered in a randomised order to ensure that judges did not evaluate the same sample at the same time. The judges were instructed to begin with the first sample on the left side of the plate and follow it clockwise. They were also asked to assess the traits according to a defined sequence. First, they had to smell the meat immediately after removing the glass top and to evaluate boar odour intensity. They were then requested to chew and taste the meat sample and evaluate boar flavour, juiciness, tenderness, bitterness and gumminess intensities and astringent properties. Before starting the sensory evaluation of the following sample, they were asked to eat bread and rinse their mouth with light black tea.

The loin samples from C, T15 and T30 pigs originating from the same litter were served on the same dish, with an extra C sample as a control sample for the R-index test. The litters were randomised between the sessions. In four sessions (n=12, two sessions per week), the LD-strips originating from four EM were offered with a 10-min interval between servings. Data were recorded with the help of the Fizz Network data acquisition system and software (Version 2.0; Biosystems, Couternon, France).

Statistical analysis

Data for growth performance, carcass characteristics and meat quality traits were analysed with the MIXED procedure of SAS. The model used included litter and experimental groups as fixed effects. The individual pig was the experimental unit for analysis of all data. Least-squares means were calculated and considered statistically significant at P⩽0.05 and tendencies were denoted at P⩽0.10 and >0.05. Pearson’s correlations between boar taint compounds and weight of testes, accessory sex glands and CYP gene isoform expression were determined using CORR procedure.

Parametric modelling of the continuous traits of the sensory analysis was performed using MIXED procedure of SAS. As residual diagnostics in the parametric linear mixed models indicated strong deviations from normality in most cases, the R package ‘robustlmm’ (Koller, Reference Koller2013) was used to estimate the model parameters by a robustified REML algorithm (Koller, Reference Koller2014). Inference was based on t-values (normal approximation), non-significant (P>0.05) interactions and (near) zero-valued variance components were step-wise excluded. The full model is given in the following equation:

(1) $$\eqalignno{Y_{{ijklm}} {\,\equals\,} & \mu {\plus}t_{i} {\plus}s_{j} {\plus}r_{k} {\plus}(ts)_{{ij}} {\plus}(tr)_{{ik}} {\plus}A_{l} {\plus}P_{m} \cr &{\plus}(tP)_{{im}} {\plus}(sP)_{{jm}} {\plus}(rP)_{{km}} {\plus}{\itε}_{{ijklm}} $$

μ is the general mean; t _i the fixed effect of treatment i; s _j the fixed effect of session j; r _k the fixed effect of service k; (ts) _ij the interaction of treatment i with session j; (tr) _ik the interaction of treatment i with service k; A _ð the random effect of animal l; P _m the random effect of panellist m; (tP) _im the interaction of treatment i with panellist m; (sP) _jm the interaction of session j with panellist m; (rP) _km the interaction of service k with panellist m; ε _iklm the residual error.

The R-indices for boar odour and flavour were computed in Excel^® according to O’Mahony (Reference O’Mahony1992) on the basis of Thurstonian modelling and signal detection theory of the categorical response values v. treatments. Inference concerning the R-indices was based on tables of critical values as published by Bi and O’Mahony (Reference Bi and O’Mahony2007).