Silage preparation

LU (Medicago sativa, cv. Sanditi), RC (Trifolium pratense, cv. Milvus), SF (Onobrychis viciifolia, cv. Perly) and two BT cultivars (Lotus corniculatus, cv. Bull (BTB) and cv. Polom (BTP)) were sown in April 2012 in Posieux, Switzerland (latitude: 46°46' N, longitude: 07°06' E, altitude: 650 m) in a field of 0.7 ha each. Each field was divided into three plots, and sampling from the plots was done at distances of ~150 m from the next sampling site, in order to obtain three independent batches (replicates) per legume. The sowing density was 26 kg/ha for LU, 23 kg/ha for RC, 160 kg/ha for SF and 30 kg/ha for BTB and BTP each. The germination rate for each legume was as follows: ⩽82% for LU, ⩽85% for RC, ⩽85% for SF, ⩽75% for BTB and ⩽75% for BTP. All legumes were cut at 1300 h at 6 cm above ground on day 73 after seeding. At that time, the SF was at the full flowering stage, whereas LU, RC, BTB and BTP were at the early flowering stage. The weed proportions in the swards were 10%, 14%, 8%, 49% and 49% of harvested biomass for LU, RC, SF, BTB and BTP, respectively. Weeds included Plantago media and Stellaria media. Sward samples were taken from each legume directly after cutting and after 24 h of wilting. The wilted samples were chopped into 1 to 2 cm pieces with a chaff cutter (Mex GT; Poettinger, Grieskirchen, Austria) and ensiled without additives in silo containers (one 0.5 l, three 1.5 l and one 30 l container/batch and per legume). The silos were covered airtight and stored in a dark room at room temperature. The dry matter (DM) losses were determined by weighing the 1.5 l silos every week on a scale (ID1; Mettler Toledo, Greifensee, Switzerland) and additionally corrected for losses due to evaporation of volatile compounds and respiratory processes according to Weissbach and Kuhla (Reference Weissbach and Kuhla1995). On day 3, the 0.5 l silos were opened for pH determinations.

After 86 days, the remaining silos were opened. Silage material from the 1.5 l silos was pooled by batch, and two subsamples were taken to determine silage characteristics and protein fractions. The silage material contained in the 30 l silos was subdivided: one part was vacuum packaged and stored at −20°C until used for the in vitro incubation. The remaining part, the fresh and wilted material collected before ensiling and one subsample from the 1.5 l silos were lyophilised (Christ, Osterode, Germany) for later analysis of the chemical composition.

Laboratory analysis of the silages

Silage pH was determined by inserting an electrode (No. 6.0202.110; Metrohm Schweiz AG, Zofingen, Switzerland) connected to an ion metre (pH/ionmeter 692; Metrohm Schweiz AG) into the filtered fluid extracted from 40 g samples shaken for 30 min with 400 ml of distilled water. The NH₃ content of each extract was also determined with an NH₃ electrode (No. 6.0506.010; Metrohm Schweiz AG).

Solutions of ~10 g silage, 90 ml distilled water, 2.5 ml Carrez I (18 g K₄Fe(CN)₆×3·H₂O in 500 ml distilled water) and 2.5 ml Carrez II (36 g ZnSO₄×7·H₂O in 500 ml distilled water) were shaken and extracted for 3 h to determine the volatile fatty acids (VFA) and short-chain alcohol contents. The acetate, propionate, butyrate, iso-butyrate, valerate, iso-valerate, lactate, propanol, propanediol, butanediol, butanol and ethanol contents of the extracts were analysed by HPLC (Summit1; Dionex, Dublin, Ireland) equipped with a nucleogel ION 300 OA 300×7.8 mm column (Macherey-Nagel GmbH, Düren, Germany) and a Shodex RI-101 refractive index detector (Shodex, Munich, Germany).

The lyophilised samples were milled to pass a 1.0 mm sieve (Brabender mill; Brabender, Duisburg, Germany). The DM was quantified gravimetrically by heating for 15 h at 60°C followed by 3 h at 105°C. The DM values were corrected for losses due to the evaporation of volatile compounds and respiratory processes according to Weissbach and Kuhla (Reference Weissbach and Kuhla1995). Organic matter (OM) was calculated from the amount of DM and total ash, which was determined by dry-ashing for 4 h at 550°C (Association of Official Analytic Chemists (AOAC), 1995; procedure no. 942.05). An ANKOM 200/220 Fiber Analyzer (ANKOM Technology Cooperation, Fairport, NY, USA) was used for NDF and ADF analysis according to standard protocols (AOAC, 1995; procedure no. 973.18 for ADF and procedure no. 2002.04 for NDF) where NDF was analysed with heat stable amylase and sodium sulphite. Both NDF and ADF were expressed without residual ash (determined by 1 h of incineration). Total N was analysed using the Kjeldahl method (AOAC, 1995; procedure no. 988.05), and CP was calculated as 6.25×N.

The total, soluble, protein-bound and fibre-bound CT contained in the SF, BTB and BTP silages were analysed using the HCl–butanol method described by Terrill et al. (Reference Terrill, Rowan, Douglas and Barry1992). In brief, for the first extraction to determine the soluble CT, ~0.5 g ground plant material DM was mixed with an acetone : water solution (7 : 3, v/v) containing ascorbic acid (1 g/l) and diethyl ether. After mixing and centrifugation, the aqueous phase was collected and concentrated. The solid residue containing the insoluble CT fraction was treated with a mix of SDS and 2-mercaptoethanol, heated for 45 min at 95°C and then centrifuged for 15 min at 25 000× g. After centrifugation, the supernatant was used to determine the amount of protein-bound CT, and the solid residue was kept to determine the amount of fibre-bound CT. The soluble and protein-bound fractions were heated with a HCl–butanol solution (5 : 95, v/v). The fibre-bound fraction was heated with a HCl–butanol solution (5 : 95, v/v) and SDS-2-mercaptoethanol. After colour development, its intensity was measured with an absorbance spectrometer (Lamda 40; Perkin Elmer Instruments, Waltham, MA, USA) at 550 nm. Standards for concentration of CT were prepared from fresh samples of SF, BTP and BTB by extraction of the CT with an acetone : water solution (7 : 3, v/v) containing ascorbic acid (1 g/l), followed by purification on a Sephadex LH-20 column (Sigma Aldrich, St. Louis, MO, USA). With these extracts, calibration curves were determined. Total phenolic compounds were analysed according to Salminen and Karonen (Reference Salminen and Karonen2011) and were expressed as gallic acid equivalents. The amounts of non-protein N (A), true soluble protein (B₁), neutral detergent soluble protein (B₂), protein insoluble in neutral detergent but soluble in acid detergent (B₃) and protein insoluble in acid detergent (C) were determined using a modified Kjeldahl method, as described by Licitra et al. (Reference Licitra, Hernandez and Van Soest1996).

In vitro incubation

The Hohenheim Gas Test, developed by Menke and Steingass (Reference Menke and Steingass1988), was used as an in vitro batch culture system. An amount of fresh silage material (single or 1 : 1 mixtures) equivalent to ~200 mg DM of the CT-containing legumes (SF, BTB, BTP) and either LU or RC were incubated separately for each batch in six runs performed on different days. Due to liquid leakage and oxygen entry, the incubation failed for some pistons, which ultimately resulted in an average of five repetitions per batch. Before incubation, the samples were ground to ~5 mm using a Moulinex food processor (Moulinex, Glattpark, Switzerland).

Ruminal fluid was collected before morning feeding from a ruminally cannulated Brown Swiss cow receiving grass hay for ad libitum intake. The cow was housed and cared for according to the Swiss legislation for animal welfare (https://www.admin.ch/opc/de/classified-compilation/20080796/index.html). The ruminal fluid was filtered through four layers of gauze and directly mixed with a preheated buffer solution (1 : 2, v/v; Menke and Steingass, Reference Menke and Steingass1988), which was flushed with CO₂ before use. Each modified piston (Soliva and Hess, Reference Steingass and Südekum2007) was filled with 30 ml of the incubation fluid, closed airtight and incubated for 24 h at 39°C in an incubator with a slow rotation. After 8 h of incubation, the gas volume was read from the calibrated scale printed onto the piston. When it exceeded 50 ml, a 0.150 ml sample was removed through an airtight septum with a sampling injector syringe (Hamilton Company, Reno, NV, USA), and the residual gas was released directly afterwards.

As CH₄ was not produced linearly during the incubation period, its concentration was directly measured in the gas from the syringes using a gas chromatograph (5890, series II; Hewlett Packard, Avondale, PA, USA) equipped with a 2.34 m×2.3 mm column (mesh size 60/80; Fluka Chemie AG, Buchs, Switzerland) and a flame ionisation detector. After 24 h, the incubation was stopped by removing the pistons from the incubator and the gas volume was recorded. The corrected total gas production was calculated as described by Menke and Steingass (Reference Menke and Steingass1988) after taking gas produced by blanks and standard samples into account. Total CH₄ production was calculated with the gas volume and concentrations measured at 8 and 24 h of incubation. It was corrected by the blank samples where the same procedure was applied.

The fluid and the incubation residue were released through the outlet of the piston, and a 10 ml volume of the fluid was collected, mixed with 0.2 ml of 50% H₂SO₄ and immediately frozen at −20°C for later analysis of total and individual VFA, as described for the silage samples. In addition, 500 μl of the incubation fluid was mixed with 500 μl of 6% formalin for microscopy determination of the total counts of Holotrich and Entodiniomorph protozoa cells using a Bürker counting chamber (0.1 mm depth; Brand GmbH & Co. KG, Wertheim, Germany). The remaining fluid and the residue were centrifuged together at 20 000×g for 30 min at 4°C. The resulting supernatant was used for pH and NH₃ determination with the appropriate electrodes (pH, HI 223; Hanna Instruments Switzerland AG, Sursee, Switzerland; for NH₃, No. 6.0506.100, Metrohm Schweiz AG). The NH₃ electrode was connected to a potentiometer (model 632; Metrohm Schweiz AG).

Calculations and statistical analysis

The uCP content of the single silages and mixtures was calculated as described by Steingass and Südekum (Reference Soliva and Hess2013) using the following formula:

$${\rm uCP}\,{\rm {\equals}}\,\left[ {{\rm (NB{\plus}NL}{\minus}{\rm NI)}\,{\rm {\times}6}{\rm .25}} \right]{\rm /\!(IW{\times}DM)}$$

where NB is the average NH₃–N concentration of the blanks, NL the N content of the silage sample, NI the NH₃–N concentration of the incubation fluid after 24 h and IW the initial weight of the incubated silage sample. The values of the silage quality and chemical composition were averaged over the three batches per legume, and the means are displayed in the tables. The protein fraction data were subjected to ANOVA using the MIXED procedure of the SAS 9.2 software with treatment as fixed effects. Multiple comparisons among means were calculated using Tukey’s procedure.

Explorative graphics and residual analyses of parametric models led to the decision to apply non-parametric inferential methods for the data obtained from the in vitro incubation. The focus of the study was on the treatment comparisons of the single legumes and the mixtures and on the comparison of the single legumes with the respective mixtures; therefore, rank-based ANOVA (Kruskal–Wallis tests) and pairwise comparisons of treatments (Wilcoxon–Mann–Whitney tests) were applied at the significance level of P<0.05 using the statistical package of the R 3.1.2 program (R Core Team, Reference Patra and Saxena2014). The different batches were treated as replicates for the respective legumes. This resulted, on average, in 15 incubations/legume (n=15). The means were trimmed at 10%, and the pooled standard errors of the means are displayed in the tables.