Animals and experimental treatments

Four primiparous lactating Holstein cows fitted with ruminal cannulas (10 cm; Bar Diamond Inc., Parma, ID, USA) were used in a 4 × 4 Latin square design with four 21 d periods balanced for residual effect and four treatments. The cows averaged 92 (se 12) d in milk at the start of the experiment with an average body weight of 575 (se 25) kg and an average body condition score of 3·00 (se 0·15; five-point scale)⁽Reference Edmonson, Lean and Weaver²⁷⁾. No antibiotics were given for at least 16 weeks before the initiation of the experiment. The cows were kept in individual stalls and had free access to water. Cows were milked twice per d at 08.30 and 20.00 hours. All cows were fed for ad libitum intake (10 % refusals on as-fed basis) twice per d (08.30 and 14.30 hours). The diet (Table 1) was formulated to meet requirements for cows that were 575 kg body weight and producing 35 kg milk/d with 3·8 % fat⁽²⁸⁾. National guidelines for the care and use of animals were followed as recommended by the Canadian Council on Animal Care⁽Reference ED, BM and AA²⁹⁾ and all experimental procedures were approved by the local Animal Care Committee ‘Comité Institutionnel de Protection des Animaux’.

Table 1 Ingredients and chemical composition of the total mixed diet

* Contained 20 % of rapeseed meal, 30 % of maize gluten meal, 20 % of soyabean meal and 30 % of brewer's corn.

† The premix contained (per kg diet): 2·3 g Ca; 1·2 g P; 1·2 g Mg; 0·4 g S; 3·5 g Na; 0·4 g K; 51·7 mg Fe; 68 mg Zn; 11·2 mg Cu; 45·4 mg Mn; 1·7 mg I; 0·2 mg Co; 0·5 mg Se; 113 00 IU vitamin A (118·4 μmol/l); 1450 IU vitamin D₃ (90 480 nmol/l); 67 300 IU vitamin E (1048 796 μmol/l).

‡ Calculated using published values of feed ingredients⁽²⁸⁾.

The four experimental treatments were: (1) oil and hulls administered in the abomasum (ABO/ABO); (2) oil placed in the rumen and hulls administered in the abomasum (RUM/ABO); (3) oil and hulls administered in the rumen and abomasal infusion of water (RUM/RUM); (4) oil infused in the abomasum and hulls placed in the rumen (ABO/RUM). Abomasal infusions consisted of 20 kg tap water (RUM/RUM treatment), 400 g flax oil+20 kg tap water (ABO/RUM treatment) or 1800 g flax hulls suspended in 18·2 kg tap water (ABO/ABO and RUM/ABO treatments). Flax oil (Brenntag Canada Inc., Montreal, QC, Canada) contained (expressed as a percentage of total fatty acids): 16 : 0, 5·3 %; 18 : 0, 3·8 %; cis-9–18 : 1, 18·4 %; cis-11–18 : 1, 0·8 %; cis-9, cis-12–18 : 2, 15·8 %; cis-9, cis-12, cis-15–18 : 3, 52·7 %; others, 3·2 %. Flax hulls (Natunola Health Inc., Nepean, ON, Canada) contained (expressed as a percentage of DM): crude protein, 23·5 %; neutral-detergent fibre, 19·4 %; acid-detergent fibre, 14·3 %; total lipids, 29·8 %; SDG, 0·99 %; 6·86 kJ/g DM. During the first 7 d of each 21 d period, only 30 % of the experimental dose of oil and hulls was administered in the abomasum over a 7 h period. From day 8 to day 21, infusion in the abomasum was conducted with 100 % of the experimental dose of oil and hulls over a 23 h period. Administration in the rumen was done by adding one-third each of oil and hulls three times daily (09.30, 14.30 and 21.30 hours) during all the experiment. Samples of the diet and of flax hulls were taken daily from day 14 to day 21 and pooled within period. All samples were frozen at − 20°C for subsequent drying at 55°C and analysed according to the procedures used by Petit & Benchaar⁽Reference Petit and Benchaar³⁰⁾. Infusates of flax products were prepared daily and the appropriate amount of infusate for each cow was weighed into tared buckets that were stirred continuously while being infused. To perform abomasal infusions, an infusion line was inserted through the rumen cannula and the sulcus omasi into the abomasum as described by Gressley et al. ⁽Reference Gressley, Reynal and Colmenero³¹⁾. Placement of the infusion lines was monitored daily to ensure post-ruminal delivery. Suspensions were pumped into the abomasum by using peristaltic pumps (Masterflex L/S; Cole-Parmer Canada Inc., Montreal, QC, Canada). The daily amount of oil supplied by flax hulls was similar to that supplied by flax oil. Half of the lipids were provided by flax oil and the other half by flax hulls for a total amount of 800 g daily, thus resulting in a fat intake below 6 to 7 % of the DM, which is known to have little effect on DM intake⁽²⁸⁾.

Sampling

Feed intake and milk yield were measured daily. Milk samples were taken twice daily from day 16 to day 21, pooled on a 6 d basis proportionally to the corresponding milk yield, and frozen at − 20°C for lignan analysis. On day 20, blood was withdrawn into K₃EDTA-vacutainer tubes (Becton Dickinson and Cie, Rutherford, NJ, USA) from the jugular vein 6 h after the morning meal. Plasma samples were kept frozen at − 20°C until lignan analysis. On day 21, a sample of urine was taken 2 h after the morning meal by hand stimulation of the perineal region and kept frozen at − 20°C for lignan analysis. Also, ruminal contents were collected 0, 2, 4 and 6 h after the morning meal from different locations within the rumen (the anterior dorsal, anterior ventral, medium ventral, posterior dorsal and posterior ventral locations) to obtain a representative sample. Ruminal pH was monitored immediately after sample collection with a portable pH meter (Oakton; Eutech Instruments Pte Ltd, Singapore). The ruminal contents were then strained through four layers of cheesecloth. A 350 ml sample of strained ruminal fluid was mixed with ruminal retentate (26 g) and frozen at − 20°C until assay for β-glucuronidase activity. One portion of filtered ruminal fluid was acidified to pH 2 with 50 % H₂SO₄ and frozen at − 20°C for later determination of volatile fatty acids (VFA) and ammonia-N concentrations. Concentrations of NH₃ and VFA in ruminal fluid were analysed, respectively, with the indophenol-blue method⁽Reference Novozamsky, Van Eck and Van Schouwenburg³²⁾ and a GLC Waters Alliance 2695 system (Waters, Milford, MA, USA) fitted with an IR detector autosampler according to the procedure used by Petit & Benchaar⁽Reference Petit and Benchaar³⁰⁾. Another portion of ruminal fluid was kept at − 20°C and freeze-dried for further analysis of lignans. As previous results (N Gagnon, C Côrtes, D da Silva, R Kazama and HV Petit, unpublished results) have shown that there is no variation in ruminal lignan concentration after feeding, ruminal samples for the three post-feeding times (2, 4 and 6 h) were pooled within cow and period to obtain only one composite sample for lignan analysis. Moreover, faecal grab samples (250 g) were collected directly from the rectum 2, 4, 6 and 8 h post-feeding on the same day (day 21). Faecal pH was monitored immediately after sample collection. Faecal samples were pooled and kept frozen at − 20°C for further β-glucuronidase analysis.

Lignan extraction

Lignans in ruminal fluid, plasma, urine and milk samples were hydrolysed and extracted according to the method of Frank & Custer⁽Reference Frank and Custer³³⁾ with some modifications. Freeze-dried samples of filtered ruminal fluid were re-suspended in Milli-Q purified water (20 mg/0·5 ml) as described by Heinonen et al. ⁽Reference Heinonen, Nurmi and Kiukkonen³⁴⁾. A quantity of 500 μl warmed (40°C) milk and re-suspended ruminal samples (0 h and pooled post-feeding samples) were mixed with 5 μl β-glucuronidase/arylsulfatase from Helix pomatia (Roche-Diagnostics, Laval, QC, Canada) while 500 μl plasma and urine were mixed with 500 μl 0·1 m-sodium acetate buffer (pH 5) and 5 μl β-glucuronidase/arylsulfatase. Milk samples were incubated for 1·5 h while plasma, urine and ruminal samples were incubated overnight at 37°C in a shaking water-bath. After hydrolysis, all samples were acidified with 10 μl 6 m-HCl. Acidified milk samples were washed with 3 ml hexane before extraction to remove lipids⁽Reference Raffaelli, Hoikkala and Leppälä¹⁹⁾. All samples were extracted with 2 ml diethyl ether. The samples were vortex-mixed twice for 2 min. The organic layer was separated by freezing. The remaining liquid phase was submitted to a second extraction under the same conditions. The organic layers were pooled and evaporated by vacuum (Speed-Vac; Thermo Savant, Holbrook, NY, USA) at room temperature for 40 min. The dry extract was re-dissolved in 500 μl enzyme immunoassay (EIA) buffer and warmed at 37°C. Four serial dilutions were done in EIA buffer for EL analysis using an EIA kit (Cayman Chemical, Ann Arbor, MI, USA). The starting dilutions were 1:50, 1:200, 1:1600 and 1:60 000 for milk, plasma, ruminal fluid and urine samples, respectively. The kit is a competitive assay that recognises both enantiometric forms of EL and utilises a standard curve ranging from 15·6 to 2000 pg/ml. The assay exhibits a limit of quantification (defined as 80 %B/B₀; 80% binding of samples) of 70 pg/ml and a half-maximal inhibitory concentration (IC₅₀; 50 % B/B₀) of 240 pg/ml. The recoveries of EL ranged from 85 to 104 %.

β-Glucuronidase activity

The determination of β-glucuronidase activity was based on a modified method of Jenab & Thompson⁽Reference Jenab and Thompson¹⁸⁾. Briefly, faecal samples (5 g) were homogenised with a Polytron (Kinematica AG, Lucerne, Switzerland) in a final volume of 20 ml cold KH₂PO₄ (pH 6·8) for 15 s while ruminal samples were homogenised using a stomacher (A. J. Seward & Co. Ltd, London, UK). Samples were then filtered through two layers of cheesecloth, sonicated on ice (two bursts, 1 min; Sonics and Materials Inc., Danbury, CT, USA) and centrifuged at 10 000 g for 15 min at 4°C. The supernatant fraction was stored at − 80°C until enzyme assay. Activity of the β-glucuronidase was quantified by mixing 25 μl of extracted sample with 125 μl 0·04 m-KH₂PO₄ (pH 6·8), 50 μl 0·5 mm-EDTA and 50 μl 5 mm-phenolphthalein diglucuronide (Sigma-Aldrich, Oakville, ON, Canada). The assay was performed in quadruplicate with one duplicate used as a baseline and the other one was incubated at 37°C for 60 min. The reaction was stopped by adding 1·25 ml 0·2 m-glycine buffer (pH 10·4) containing 0·2 m-NaCl. After 10 min of incubation at room temperature, 200 μl of each replicate was transferred to a ninety-six-well flat-bottomed plate and the plate was read on a Spectra Max 250 ELISA reader (Molecular Devices, Sunnyvale, CA, USA) at 540 nm. The absorbance values directly correlate to the amount of the phenolphthalein released based on a phenolphthalein standard curve. The specific activity of β-glucuronidase was calculated by the formula: (nmol phenolphthalein 60 min – nmol phenolphthalein 0 min)/(60 min × mg protein). Protein was determined by a bicinchoninic acid protein assay kit (Sigma-Aldrich) using bovine serum albumin as the standard.

Statistical analysis

All data were analysed using the MIXED procedure of SAS (SAS 2000; SAS Institute, Cary, NC, USA) according to the model:

where Y_ijk is the response variable, μ is the overall mean, a_i is the random effect of cow i, β_j is the effect of period j, τ_k is the effect of treatment k and e_ijk is the residual error. The residual effect was initially included in the model but was removed because it was not significant. Data on EL concentrations were transformed (log) as previously performed by Hausner et al. ⁽Reference Hausner, Johnsen and Hallund³⁵⁾ and Nesbitt et al. ⁽Reference Nesbitt, Lam and Thompson³⁶⁾ but the results in Table 2 are reported as the adjusted mean value (with CI) on the original scale of measurements. The model for specific β-glucuronidase activity and pH was augmented with time and time × treatment interaction for repeated measurements and values are reported with their adjusted mean values with standard errors. The two-sided level of significance was set at P < 0·05, although probability values up to P < 0·1 are shown in the text if the data suggest a trend. When a significant F test was detected, multiple comparisons were done using a Tukey's adjustment for the probability. A specific contrast was also used a posteriori to compare the site of administration of either oil or hulls.

Table 2 Concentration of enterolactone in biological fluids of Holstein cows receiving oil and hulls administered in the abomasum (ABO/ABO), oil placed in the rumen and hulls administered in the abomasum (RUM/ABO), oil and hulls placed in the rumen (RUM/RUM) and oil infused in the abomasum and hulls placed in the rumen (ABO/RUM)

(Adjusted mean values and 95 % confidence intervals on the original scale of measurements)

^a,b Mean values within a row with unlike superscript letters were significantly different (P < 0·05).