Experimental design, animals and diets

The experiment described in the present paper was part of a larger study on starch digestion kinetics, which is described in detail elsewhere^{(Reference Martens, Flécher and de Vries26)}. The experiment was approved by the Dutch Central Committee of Animal Experiments under the authorisation number AVD260002016550. Briefly, ninety crossbred gilts (Topigs 20 × Pietrain sire), weighing 23·1 (sd 2·0) kg, were assigned to one of the nine dietary treatments in a 3 × 3 factorial arrangement, in four successive batches. Factors were starch source (barley, maize and high-amylose (HA) maize) and form (isolated starch, ground cereal and extruded cereal). The resulting dietary treatments were: barley starch in isolated (IB), ground (GB) and extruded (EB) forms; maize starch in isolated (IM), ground (GM) and extruded (EM) forms and HA maize starch in isolated (IA), ground (GA) and extruded (EA) forms. In total, ninety-six pigs were used: ten pigs were assigned per dietary treatment, whereas the remaining animals served as reserve animals and were used to replace excluded animals. Fourteen pigs were excluded due to a low feed intake: pigs that were excluded in one of the first three batches were replaced in the sequential batch. Replacement was done in such a way that a minimum of seven observations was realised for each dietary treatment. The experiment consisted of an adaptation period of at least 2 d, followed by an experimental period of at least 12 d, during which the experimental diets were fed. Pigs were housed in groups of four animals per pen but fed individually at 2·0 × the energy requirements for maintenance (750 kJ net energy per kg body weight^0·60)⁽²⁷⁾, divided over two equal meals at 08.00 and 16.00 hours. All the diets were mixed with water just before feeding. In the first batch, all diets were mixed with water to a feed:water ratio of 1:2. After the first batch, the feed:water ratio of ground diets was altered to 1:1·5 to facilitate ingestion. Pigs always had free access to water. During the last 2 d of the experimental period, the daily allowance of the pigs was equally divided over six meals, starting at 07.00 hours and applying a between-meal interval of 3 h, to reach a constant passage rate of digesta through the GIT. Just prior to dissection, a frequent feeding procedure was applied to enable the measurement of digesta passage kinetics: Each pig was fed six meals containing 1/12th of their daily allowance each, applying a 1-h between-meal interval. The first of the six hourly meals was fed exactly 6 h before a pig was euthanised. Pigs were euthanised and dissected in an order balanced for dietary treatment and time after onset of the frequent feeding procedure. Upon the start of the frequent feeding procedure of the first pig, extra meals (1/12th of daily feed allowance) were provided with 2-h intervals to the pigs whose frequent feeding procedure had not yet started, to prevent restlessness in the barns. Diets were formulated to meet or exceed the nutrient requirements of growing pigs⁽²⁷⁾ and designed to contain about 400 g starch per kg dry feed. All diets were formulated to be identical in crude protein, fat and total dietary fibre content, using soyabean meal, soyabean hulls, soyabean protein isolate, soyabean oil and sugar beet pulp. Details on ingredients, production conditions and the analysed composition are described elsewhere^{(Reference Martens, Flécher and de Vries26)}. Cr and Co were included as markers in the feed at a level of 170 mg/kg to study digesta passage behaviour of solid and liquid digesta fractions, respectively. Cr was included in the form of chromium oxide (Cr₂O₃) and Co was included in the form of Co-EDTA.

Digesta collection

Prior to dissection, pigs were sedated and exsanguinated as described in detail elsewhere^{(Reference Martens, Flécher and de Vries26)}. Immediately after exsanguination, clamps were placed between gastrointestinal sections to prevent the movement of digesta and the GIT was carefully removed. The stomach content was homogenised by manual mixing, and after recording the total weight and the pH, samples were collected. One representative sample was immediately frozen and kept at −20°C until freeze-drying, whereas another sample was kept at 4°C pending rheology and particle size analyses. The SI was carefully spread on a table and divided with clamps in four segments. The last 1·5 m from the SI (SI4) was considered to represent the terminal ileum. The rest of the SI was divided in three parts with equal length (SI1, SI2 and SI3, from proximal to distal SI). All parts were dissected, and their contents were collected by gentle stripping after which digesta of each part were manually homogenised. The total weight of the digesta was recorded, and a representative sample was immediately frozen and kept at −20°C until freeze-drying. In addition, samples from SI2 and SI4 were taken and stored at 4°C pending rheology and particle size analyses.

Chemical, physical and rheological analyses

Prior to chemical analyses, feed and freeze-dried digesta samples were ground to pass a 1 mm sieve using a centrifugal mill at 12 000 rpm (ZM200; Retsch). All analyses were performed in duplicate, unless indicated otherwise. DM content of digesta was determined in singlicate by recording the weight before and after freeze-drying. DM content in feed was determined according to NEN-ISO 6496⁽²⁸⁾.

Viscosity of digesta was measured using stress-controlled rheometers (MCR 301/MCR 502, Anton Paar GmbH) in samples (<48 h after digesta collection, stored at 4°C), without separation of the liquid and solid fraction and without grinding the samples, at 39°C. Samples were analysed as described previously^{(Reference Shelat, Nicholson and Flanagan15)}, with slight adjustments. Briefly, feed samples were analysed after soaking the feed for 1 h in the feed:water ratio as fed from batch 2 onwards (1:2 for diets with isolated starch and extruded cereals, 1:1·5 for diets with ground cereals). A parallel plate profiled geometry (PP25/P2) of 25 mm diameter with a ribbed surface was used to avoid slip, and a plastic lid was used to avoid evaporation. For small intestinal digesta samples, harvested from the second and last part of the SI, the apparent viscosity curve was measured using a frequency sweep (100–1 Hz log). Feed and stomach digesta had both solid and liquid properties. To ensure permanent contact and confinement pressure, those samples were subjected to an oscillatory frequency sweep (from 275 to 1 Hz) at normal force controlled gap distance (0·5 N) and a constant strain (10 %). Settings were optimised based on the sample that had visually the highest gel strength, which was stomach digesta originating from pigs fed diets with isolated starch. For stomach digesta recovered from pigs fed EB or EM, the gel strength was not sufficient to remain a constant normal force controlled gap distance. Therefore, samples were subjected to the oscillatory frequency sweep at a fixed gap distance (2 mm). With the oscillatory measurements, we identified the shear stress, storage modulus (G′) and loss modules (G″) at a frequency of 1 Hz, as previous research suggested that the forces naturally applied by the GIT are close to this frequency^{(Reference Donnelly, Jackson and Ambrous29–Reference Lentle, Hemar and Hall31)}.

Particle size of digesta was analysed at 20°C in samples that were stored at 4°C or −21°C. Feed samples were analysed after soaking for 1 h in the feed:water ratio as fed from batch 2 onwards (1:2 for diets with isolated starch and extruded cereals, 1:1·5 for diets with ground cereals). Particle size was measured by laser diffraction (Mastersizer 3000; Malvern) using demineralised water as a dispersant. The reference material was wood flour (refraction index 1·53, absorption index 0·1, as supplied by the manufacturer), and each sample was analysed at least in triplicate. Measurements were performed in the range of 0·01–3500 μm. For further analyses, the volume percentage of particles was summarised in three classes: small particles, between 3·5 and 35 µm; medium particles, 35–350 µm and large particles, 350–3500 µm.

WHC of diets and freeze-dried digesta was determined in ground material using Baumann’s apparatus^{(Reference Baumann32)}. A total of 105 (sd 6) mg of ground and freeze-dried samples was placed on a filter disc of 40 mm diameter with 10–16 µm pore size (Duran group). The volume of water absorbed to hydrate the sample until saturation was recorded and corrected for the amount of water that evaporated in this time, which was determined using a filter disc without sample.

Cr and Co concentrations were measured in singlicate by inductively coupled plasma optical emission spectroscopy. Cr and Co were measured at 357·9 and 228·0 nm, respectively, according to Van Bussel et al.,^{(Reference van Bussel, Kerkhof and van Kessel33)} after sample preparation according to Williams et al.^{(Reference Williams, David and Iismaa34)}

Molecular weight distributions of the soluble fractions of feed and digesta were analysed with high-performance size exclusion chromatography (HPSEC). Digesta from all pigs within a dietary treatment were pooled by mixing equal weight aliquots of freeze-dried digesta of each pig. Freeze-dried and ground diets and pooled digesta were boiled in water for 5 min (50 mg/ml) and subsequently centrifuged. Supernatant was analysed using an Ultimate 3000 HPSEC system (Thermo Fisher Scientific). A set of four TSK-Gel columns (Tosoh Bioscience) was used in series: one guard column (6 mm inner diameter × 40 mm) and the columns super AW4000, 3000 and 2500 (6 mm inner diameter × 150 mm). The column temperature was set to 55°C. A volume of 10 μl of sample was eluted with filtered 0·2 M NaNO₃ at a flow rate of 0·6 ml/min, and the elution was monitored by refractive index detection (Shodex refractive index 101; Showa Denko K.K.).

Calculations and statistical analyses

The MRT of solid and liquid fractions of digesta was calculated based on quantities of Cr and Co recovered in GIT segments, assuming that hourly feeding induced steady-state conditions, according to Equation 1^{(Reference de Vries, Gerrits, Moughan and Hendriks35)}:

$${\rm{MRT}}\left( n \right) = \left( {300 \times \left[ {{\rm{marker}}} \right] \times W} \right)/I$$ (1)

Where MRT is the mean retention time in minutes in compartment n of the GIT; [marker] is the marker (Cr or Co) concentration in the digesta (mg/g DM); W is the weight of the dry intestine content (g DM) and I is the marker intake over 300 min prior to dissection (mg). ΔMRT was calculated as digesta MRT of solids minus the digesta MRT of liquids at each GIT compartment.

The power law model was used to model the apparent viscosity of small intestinal digesta, per pig per segment, measured over a range of shear rates (Equation 2)^{(Reference Holdsworth36)}:

$${\rm{Apparent\;viscosity}} = K \times {\rm{shearrat}}{{\rm{e}}^{\left( {n - 1} \right)}}$$ (2)

where K is the consistency coefficient (Pa*sⁿ), which reflects the shear stress at a shear rate of 1/s, and n is the flow behaviour index, which is dimensionless and reflects the closeness to Newtonian flow. K and n were estimated by nonlinear regression procedures (PROC NLIN, SAS, version 9.4, SAS Institute).

To characterise the rheological properties of diets and stomach digesta, tanδ was calculated according to Equation 3^{(Reference Mezger and Mezger37)}:

$$tan\delta = {\frac{{{\rm{Loss\;modulus}}}}\over{{{\rm{Storage\;modulus}}}}}$$ (3)

where loss and storage moduli were measured at 1 Hz.

From the DM content and WHC of diets and digesta, we calculated the saturation ratio (SR). The SR is the digesta water content, as fraction of the theoretical maximum of water that can be held by the DM according to its WHC. The SR was calculated according to Equation 4:

$${\rm{SR}} = {\frac{{{\rm{Water\;content}}}}\over{{{\rm{Max\;water\;held}}}}}$$ (4)

Where the water content is the percentage of water in the dietary or digesta suspension and max water held is the amount of water that can maximally be held in the dietary or digesta suspension, calculated as the DM content times WHC. For diets, the water content represents the water content of diets after they were mixed with water, in the ratios applied prior to feeding. An SR < 1 indicates that less water is present in the stomach than the amount of water that can potentially be held by the amount of DM. An SR > 1 indicates that more water is present in the stomach than can be held by the digesta matrix, based on its WHC properties.

Effects of dietary treatments on MRT were tested using a general linear mixed model (PROC MIXED, SAS), with starch form, starch source and their interaction as fixed effects and batch as random effect. Least square means were compared after Tukey’s adjustment for multiple comparisons. Correlation coefficients between whole digesta rheology parameters and MRT, and whole digesta rheology and physical properties, were estimated using Pearson’s correlation procedure (PROC CORR, SAS). Data are presented as least squares (LS) means and pooled standard deviation of the mean (S) unless stated otherwise. A retrospective power analysis was performed to validate the sample size of the present study. Considering digesta MRT as the most important parameter, the power was evaluated using the variation in digesta MRT observed in the present study, by calculating the critical F-value for a two-sided a level of 0·05 and for the mixed model study design^{(Reference Stroup38)}. For the stomach and SI, a power >0·69 was reached on the main effect of starch form and a power >0·52 was reached on the main effect of starch source. For the form × source interaction, a power of 0·29 was reached for the stomach and a power of 0·72 was reached for the SI. Significance was assumed at P ≤ 0·05, while a tendency was considered when 0·05 < P ≤ 0·1.