Animals and experimental design

The study was conducted at the Experimental Research Station of Universidad Austral de Chile, Valdivia, Chile, between January and March 2017.

Twelve pregnant multiparous lactating Holstein Friesian dairy cows (mean ± Standard error: 22.7 ± 0.67 kg milk/day, 534 ± 7.5 kg liveweight and 155 ± 6.6 days in milk) were randomly allocated to three dietary treatments in a replicated 3 × 3 Latin square design. The experiment lasted 63 days and was divided into three 21-day periods each; the first 14 days of each period consisted in adaptation of the animals to the diets and the last 7 days were used for data collection. Seven days before the first experimental period, the cows were housed in tie-stalls with rubber bedding for adaptation to experimental conditions and received a grass silage and concentrate diet.

Brassica crop production and animal feeding

Turnip cv. Barkant and FR cv. Spitfire were sown in October and November 2016 in two adjacent 0.5 ha area at a density of 3 and 4 kg seed/ha, respectively. The crops were sown on two dates with a 20-day interval, in order to offer plant material with a similar stage of maturity throughout the experiment. A fresh allocation of ST was harvested manually daily and soil attached to the roots removed, whereas FR was harvested with a cutter bar mower (Bertolini 140 L, Reggio Emilia, Italy) at 10 cm above ground level daily.

Cows were divided into three groups according to the dietary treatments (control, ST and FR). For the control diet, 16.2 kg DM of grass silage, 2.25 kg DM of commercial concentrate and 2.25 kg DM soybean meal were offered on a daily basis. For the other two dietary treatments, 25% of the DM from silage and concentrates were replaced with FR (leaf : stem ratio: 65 : 35) or ST (leaf : root ratio: 46 : 54). The amount of soybean meal remained constant to keep the three diets isoenergetic and isonitrogenous, which met the ME and protein requirements based on AFRC (1995). Chemical composition of feed ingredients and diets is reported in Table 1. Prior to feeding, all feeds were weighed and offered individually for each cow according to the dietary treatments. Grass silage and soybean meal were offered twice a day at 0800 and 1700 h. Once cows consumed the soybean meal, grass silage was offered. For ST and FR, orts of grass silage were removed at 1100 h and the total allowed amounts of ST or FR were offered at once for a 5 h period. Concentrates were offered twice daily during milkings.

Table 1 Chemical composition of feed ingredients, diets (control, rape and turnip) and proportion of ingredients offered to mid-lactation dairy cows

FR = treatment with a 25% of forage rape inclusion in the diet; ST = treatment with a 25% of summer turnip inclusion in the diet; DM = dry matter (g/kg); aNDF = neutral detergent fibre with a heat stable amylase (g/kg DM); ADF = acid detergent fibre (g/kg DM); CP = crude protein (g/kg DM); NFC = non-fibrous carbohydrates (NFC = 1000 – (ash + lipid + CP + NDF) (g/kg DM); DOMD = digestible organic matter on DM basis (g/kg DM); ME = metabolizable energy (Mcal/kg DM).

Feeds and nutrients intake, milk production and composition

Feed offered and feed refusals were recorded daily. The content of DM in the feeds was determined on days 1, 3 and 5 of week 3 of each period. Sub-samples of forages (silage, ST and FR) collected once per experimental period, were freeze-dried and ground through a 1 mm screen (Wiley Mill, 158; Arthur H. Thomas, Philadelphia, PA, USA) prior to chemical analyses. Leaves and roots of ST and leaves and stems of FR were analysed separately. Leaf : root and leaf : stem ratios were determined for ST and FR, respectively. Dry matter content was determined by weighing before and after drying in a forced-air oven at 105°C for 12 h. For each sample, ash and lipids were analysed according to AOAC (1996; method 942.05 and 920.39 for ash and lipids, respectively); nitrogen (N) content was determined by combustion (Leco Model FP-428 Nitrogen Determinator; Leco Corporation, St Joseph, MI, USA) and was used to calculate CP content (N × 6.25). Neutral detergent fibre was determined as aNDF (Van Soest et al., Reference Van Soest, Robertson and Lewis1991) using heat stable amylase (Ankom Technology Corp., Macedon, NY, USA) and ADF according to AOAC (1996; method 973.18). Digestible organic matter on DM basis (DOMD) was measured according to Tilley and Terry (Reference Tilley and Terry1963) and was used to estimate ME by regression (ME = 0.279 +0.0325 * DOMD(%)) (Poff et al., Reference Poff, Balocchi and Lopez2011). Non-fibrous carbohydrates (NFCs; g/kg DM) were estimated as follows:

$${\rm{NFC = 1000}} - \left( {{\rm{ash}}\,{\rm{ + }}\,{\rm{CP}}\,{\rm{ + }}\,{\rm{lipids}}\,{\rm{ + }}\,{\rm{aNDF}}} \right).$$

Cows were milked at 0700 and 1600 h and milk yield was recorded daily with a flow sensor (MPC580 DeLaval, Tumba, Sweden) during the experimental periods. The average for the final week of each period is reported. Representative milk samples were collected at morning and afternoon milkings for 3 days in the last week of the experimental period for fat, protein, lactose and milk urea analyses by mid-IR spectrophotometry (Foss 4300 Milko-scan; Foss Electric, Hillerod, Denmark).

Rumen fermentation

Rumen fluid was harvested by stomach tubing (Flora Rumen Scoop; Prof-Products, Guelph, ON, Canada) before (1000 h) and 6 h (1600 h) after brassica supplementation on day 6 of week three in each experimental period.

Samples were strained through four layers of cheesecloth. A 10-ml sample was drawn off, mixed with 0.2 ml of 50% (wt/vol) sulphuric acid and stored at −20°C pending determination of short-chain fatty acid (SCFA) and ammonia (NH₃) concentrations. Rumen fluid was allowed to thaw for 16 h at 4°C and then centrifuged at 10 000×g for 10 min at 4°C. Six microlitres of supernatant was drawn off and then centrifuged at 10 000×g for 10 min at 4°C. Thawed supernatant of rumen fluid samples was analysed for SCFAs by gas chromatography as described by Tavendale et al. (Reference Tavendale, Meagher, Pacheco, Walker, Attwood and Subathira2005) and for NH₃ by the phenol-hypochlorite reaction method (Weatherburn, Reference Weatherburn1967). Total SCFA (tSCFA) were considered as the sum of acetate, butyrate, proportionate, isobutyrate, valerate, isovalerate and caproate. Minor SCFAs are the sum of isobutyrate, isovalerate, valerate and caproate.

For the whole experiment, rumen pH was monitored by wireless telemetric pH bolus (eCow, Exeter, UK). Before the experiment started, an internal validation of the pH bolus was conducted with three cannulated cows. The ruminal samples were collected during 2 days from three sites within the rumen (cranial, ventral and caudal) every 2.5 h. Immediately after collection of rumen fluid, pH was measured by glass electrode (Model HI98127; Hanna Instruments, Woonsocket, RI, USA). The pH boluses were calibrated before use, programmed to measure rumen pH at 15-min intervals and inserted directly into the ventral sac of the rumen of each cow. The data were transmitted wirelessly to a transceiver connected to a cell phone and then transferred to a laptop computer. The pH data were summarized as mean pH, pH per hour, time spent with pH < 6.2 and >6.0, and below pH 6.0.

Urine collection and purine derivative measurements

Spot urine samples (20 ml) were collected by vulva stimulation (Cosgrove et al., Reference Cosgrove, Jonker, Lowe, Taylor and Pacheco2017) every 3 h once a day during day 5 of week 3 in each experimental period, to estimate rumen microbial N flow based on purine derivatives (PDs, allantoin + uric acid) by HPLC. Samples were acidified with 2 ml sulphuric acid (10% v/v) to maintain pH below 3 and stored at −20°C. Urine samples were thawed, a composited sample per cow was made for each period and analysed for allantoin, uric acid and creatinine by HPLC. Urine volume was estimated using creatinine concentration as a marker (Lindberg, Reference Lindberg1989). The amount of microbial purines absorbed (PA, mmol/day) and the PD excreted was estimated from the predictive model proposed by Singh et al. (Reference Singh, Sharma, Dutta, Singh, Verma and Mehra2007) and the microbial nitrogen flow (MN, g/day) was estimated according to Makkar (Reference Makkar, Makkar and Chen2004). Full equations are presented in Supplementary Material S1.

Haematological measures

Blood samples were collected on day 4 of week 3 in each period, after morning milking. Blood was collected from a coccygeal vessel using two evacuated blood collection tubes (BD Vacutainer; Becton, Dickinson and Company, New Jersey, USA): one containing Ethylenediaminetetraacetic acid (4 ml) and one with no anticoagulant (9 ml). Samples were transported on ice to the haematology laboratory of the Universidad Austral de Chile Teaching Hospital for analysis, where they were centrifuged at 3000 × g for 10 min at 25°C. Whole blood was used for determination of complete blood count; red blood cell (RBC); white blood cell (WBC); haemoglobin concentration; packed red cell volume (PCV); mean corpuscular volume and mean corpuscular haemoglobin concentration. For evaluation of these haematologic parameters, an automated haematology analyzer (KX-21 N; Sysmex, Kobe, Japan) was used. The blood smears were stained with rapid staining (Hemacolor; Merck, Darmstadt, Germany) for a differential WBC count. Heinz-Ehrlich bodies were counted in blood smears prepared on average 5 h after sampling, using crystal violet staining, and expressed as per cent erythrocytes containing one or more inclusion bodies. Serum samples were stored at −20°C until analysed for urea and gamma-glutamyl transferase (GGT) using a Wiener Metrolab 2300 auto-analyzer (Wiener Lab., Rosario, Argentina) at 37°C, and triiodothyronine (T₃) using a validated Elisa Kit (MyBioSource, San Diego, CA, USA).

Statistical Analyses

The data were analysed using the mixed model procedure of SAS (2006; version 9.4; SAS Institute Inc., Cary, NC, USA) to account for carryover effect according to the following model:

$${{\rm{y}}_{{\rm{ijklm}}}}{\rm{ = \mu + }}{{\rm{S}}_{\rm{i}}}{\rm{ + }}{{\rm{A}}_{\left( {\rm{i}} \right){\rm{j}}}}{\rm{ + }}{{\rm{P}}_{\left( {\rm{i}} \right){\rm{k}}}}{\rm{ + }}{{\rm{T}}_{\rm{l}}}{\rm{ + }}{{\rm{C}}_{\rm{m}}}{\rm{ + }}{{\rm{e}}_{\left( {{\rm{ijk}}} \right){\rm{l}}}},$$

where y_ijklm is an observation for each dependent variables; μ is the general mean; S_i is the fixed effect of the ith treatment sequence; A_(i)j is the random effect of the jth cow in the ith sequence; P_(i)k is the fixed effect of the kth period; T_l is the fixed effect of the lth treatment; C_m is the fixed carryover effect from the previous period (C = 0, if period = 1) and e_(ijk)l is the random error. If carryover effects were not detected, a simplified model for a replicated Latin square was used:

$${{\rm{y}}_{{\rm{ijklm}}}}{\rm{ = \mu + }}{{\rm{S}}_{\rm{i}}}{\rm{ + }}{{\rm{A}}_{\left( {\rm{i}} \right){\rm{j}}}}{\rm{ + }}{{\rm{P}}_{\left( {\rm{i}} \right){\rm{k}}}}{\rm{ + }}{{\rm{T}}_{\rm{l}}}{\rm{ + }}{{\rm{e}}_{\left( {{\rm{ijk}}} \right){\rm{l}}}}$$

where y_ijklm is the observation for dependent variables; μ is the general mean; S_i is the random effect of the ith square; A_(i)j is the random effect of the jth cow in the ith square; P_(i)k is the fixed effect of the kth period; T_l is the fixed effect of the lth treatment and e_(ijk)l is the random error. The interaction of treatment and period was tested and was determined to be not significant (P > 0.05). As a result, this interaction was removed from the model. Data for DMI, milk yield, milk composition, microbial N and haematological measures were summarized by day. For haematological measures, three tubes were not reported by the laboratory due to coagulation of samples, and therefore different standard errors are reported for each treatment. Data for SCFA, NH₃ and pH were analysed with the same model but including sampling time or hour as a repeated measurement and the interaction of treatment and repeated measurement, with cow as a subject. The estimation method was REML and the df method was Kenward–Roger. The variance–covariance structure that yielded the lowest corrected Akaike information criterion was compound symmetry and selected for the final model. Values reported are least squares means and associated standard errors of the mean. Statistical significance was declared at P ≤ 0.05 and trends at 0.05 < P ≤ 0.10. The PDIFF command, incorporating the Tukey–Kramer adjustment for multiple pairwise comparisons of treatment means, was used (Supplementary Material S2).