Animals and diets

Male Wistar rats (average weight, 53·9 (sem 0·6) g) were purchased from Taconic (Bomholt, Denmark). The experiment was carried out in four blocks with twelve rats in each block during a period of 3 months. The rats were housed in pairs in Plexiglas boxes (38 cm × 60 cm) bedded with shavings. All rats had a chip placed subcutaneously in order to allow individual identification of the rats. The animals were kept in a temperature- (25–26°C) and humidity (50–60 %)-controlled environment in a 12 h light/dark cycle.

The rats were randomly assigned to one of six dietary treatments (eight rats per treatment). A FF diet was prepared according to Table 1. NDC sources were substituted for maize starch and the test diets were as follows: (1) FF; (2) C; (3) P; (4) I; (5) RS; (6) BH. The chemical composition of the diets is shown in Table 2. The concentration of NDC in the test diets was 130–152 g/kg dry diet. The diets were planned to contain the same amount of NDC. However, the amount of NDC in the various sources did deviate slightly from the expected, and hence the resulting amount of NDC in the diets differed. Inclusion of crystalline C in the diet resulted in a NDC content of 121 g/kg DM and a major part of the NDC was C. The NDC of the P diet was almost completely soluble. The source of P used (GENU^® pectin 150 USA-SAG type B rapid set) is a high-ester P with a high degree of esterification (73·5 %). The derivative of I used in the present study (Raftiline HP, Orafti, Tienen, Belgium) was a mixture of oligosaccharides with a degree of polymerisation of 3–60 (average 22–25) and the resultant content of I in the I diet was 93 g/kg DM. The NDC in the RS diet were mainly RS of the type retrograded starch and only small amounts of NSP could be detected. The BH diet contained mainly insoluble fibres, and it had the highest content of lignin.

Table 1 Composition of the experimental diets

* FF, fibre free; C, cellulose; P, pectin; I, inulin; RS, resistant starch; BH, barley hulls.

† Miprodan 25-6 (Arla Ingredients, Viby J., Denmark)+1 % methionine (Sigma-Aldrich Denmark A/S, Copenhagen, Denmark).

‡ Mineral mixture supplied the following nutrients (per kg diet): calcium citrate, 13·88 g; calcium hydrogen phosphate dihydrate, 5·08 g; potassium hydrogen phosphate, 9·85 g; KCl, 5·61 g; NaCl, 1·74 g; magnesium sulphate, 1·72 g; magnesium carbonate hydroxide pentahydrate, 1·58 g; ammonium iron(III) citrate, 0·344 g; manganese(II) sulphate monohydrate, 45 mg; copper(II) sulphate pentahydrate, 41 mg; KI, 0·225 mg; zinc sulphate heptahydrate, 99 mg; sodium selenite, 0·585 mg.

§ Vitamin mixture supplied the following nutrients (per kg diet): retinol acetate, 750 μg; dl-α-tocopherol acetate, 20 mg; menadione, 4·1 mg; choline chloride, 700 mg; folic acid, 0·7 mg; nicotinamide, 12·5 mg; calcium pantothenate, 5·0 mg; riboflavin, 2·0 mg; thiamin hydrochloride, 2·5 mg; pyridoxine chloride, 4·0 mg; cyanocobalamin, 0·03 mg; biotin, 0·25 mg; cholecalciferol, 16.25 μg.

∥ Crystalline cellulose (AGF-100, Frisenette, Knebel, Denmark).

¶ GENU^® pectin 150 grade USA-SAG type B rapid set, CP Kelco, Lille Skensved, Denmark.

** Raftiline HP^®.

†† Autoclaved potato starch.

‡‡ Axel Toft Grovvarer A/S, Roslev, Denmark.

Table 2 Analysed chemical composition of the experimental diets

* FF, fibre free; C, cellulose; P, pectin; I, inulin; RS, resistant starch; BH, barley hulls.

† N x 6·25.

‡ Non-digestible carbohydrates.

§ Not determined.

∥ Below the detection limit.

¶ Values in parentheses are soluble NSP.

Table 3 Mucin-staining area in the crypts (μm²) and the proportion of the crypt area covered with mucin (%) in the caecum and the colon of rats fed fibre-free diet (FF), cellulose (C), pectin (P), inulin (I), resistant starch (RS) or barley hulls (BH)

(Mean values with their pooled standard errors)

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

Table 4 Concentration of SCFA (μmol/g), the pool size (μmol) and the proportions of acetic, propionic and butyric acid (mol/100 mol SCFA) in the caecum and the colon of rats fed fibre-free diet (FF), cellulose (C), pectin (P), inulin (I), resistant starch (RS) or barley hulls (BH)

(Mean values with their pooled standard errors)

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

The rats were fed the experimental diets for 34–41 d. The duration of the feeding period differed because the measurements of the mucous layer were time consuming and measurements could only be performed on two rats per day, hence six working days were required to perform the measurements in each block. The rats were killed in a randomised order among the dietary treatment groups. The amount of feed was gradually increased from 12·5 g/d during the first 5 d to 20 g/d at the end of the experiment. The rats had free access to water.

The study complied with the guidelines of the Danish Animal Experiments Inspectorate, Ministry of Justice, Copenhagen, Denmark with respect to animal experimentation and care of animals under study.

Measurement of the mucous gel thickness in the colon

The rats were weighing 247 (sem 28) g when the measurement of the mucous gel thickness in the colon was performed. The measurements were carried out as previously described⁽Reference Atuma, Strugala and Allen¹⁹⁾. The rats were anaesthetised by intra-peritoneal administration of thiobutabarbital sodium (Inactin, 120 mg/kg; Sigma T-133, Sigma Chemical, St Louis, MO, USA) and subcutaneous administration of buprenorphine (Temgesic, 0·05–0·1 mg/kg; Schering-Plough, Brussels, Belgium).

The rats were tracheotomised to facilitate spontaneous breathing. The femoral vein was cannulated for the continuous infusion of 0·9 % NaCl at a rate of 1 ml/h. The rat was opened along the mid-line and the colon was identified and exteriorised. An approximately 2 cm long incision was made along the antimesenteric border. The incision was made 5·7 (sem 0·7) cm distal to the caecum. The rat was placed on its left side on a microscope stage and the colon was everted through the incision and loosely draped over a truncated cone with the luminal side up. A mucosal chamber with a hole (1·0 cm in diameter) in the bottom was placed over the exposed mucosa, and the junction was sealed with silicone grease (VWR International, Poole, England). The chamber was filled with warm (37°C) 0·9 % NaCl to keep the tissue moist and protect the mucous gel from dehydration. The mucous gel was covered with carbon particles (activated charcoal, extra pure, 1·02 184; Merck, Darmstadt, Germany) suspended in saline to visualise the surface of the otherwise near-transparent gel. A micropipette (TIP2TW1; World Precision Instruments, Hertfordshire, England) was held by a micromanipulator (MX1640R; Siskiyou Design Instruments, Grant Pass, OR, USA) and pushed into the mucous gel at an angle (α) of 30–40° to the cell surface. The distance (l) from the luminal surface of the mucous layer to the epithelial cell surface of the mucosa was measured with a digimatic indicator (543-250B; Mitutoyo, Tokyo, Japan) connected to the micromanipulator. The mucous gel thickness (T) could then be calculated from the formula T = l × sin α. The measurements were made at five different spots over the mucous surface. The procedure was carried out under observation through a stereomicroscope (Leica MZ12; Leica Microsystems AG, Wetzlar, Germany). The total mucous thickness was measured with 15 min intervals over 60 min to determine the basal mucous accumulation rate. Following these measurements, as much as possible of the mucous gel was removed by suction, and the thickness of the adherent mucous layer was determined.

Collection of digesta and tissue samples

After the termination of the mucous gel measurements, the rats were euthanised by an intra-venous injection of saturated KCl. The entire gastrointestinal tract was removed and the caecum and the colon were dissected free. The intestinal contents were collected for the determination of SCFA and tissue samples were taken for histology and mRNA determination. In order to ensure the proximity to the point where the thickness of the mucous layer was determined, the tissue sample for histology was taken cranially and the sample for the mRNA determination was taken caudally to this point. The samples for histological examinations were immediately transferred to a 4 % (v/v) neutral-buffered formalin solution (Bie & Berntsen, Rødovre, Denmark) and the samples for the mRNA determination were transferred to RNAlater ^® (R0901; Sigma), kept at 4°C for 24 h and kept at − 80°C until analysis.

Mucin staining and morphometric measurements

Intestinal segments were fixed in 4 % neutral-buffered formalin, dehydrated, cleared and embedded in paraffin. Serial sections were cut at 4 μm, deparaffinised in xylene, rehydrated and stained using a combined alcian blue–periodic acid Schiff's technique for acid and neutral mucins⁽Reference Bancroft and Gamble²⁰⁾. The slides were incubated in 5 g/l alcian blue (Sigma A3157), pH 2·5 for 15 min, then washed and incubated with 10 g/l periodic acid (Merck 524) for 5 min. After a wash in water, the slides were placed in Schiff's reagent (Merck 1.09 033). Finally, the slides were counterstained with Mayer's haematoxylin, dehydrated and mounted.

On each slide, fifteen well-oriented crypts were selected. Indicated by blue or magenta staining, the granules of all mucous cells (goblet cells and crypt secretory cells), as well as the apical secretion of these cells, were differentiated into acidic and neutral mucin, respectively⁽Reference Bancroft and Gamble²⁰⁾. For each crypt, the area of mucin granules with a clear positive reaction for neutral or acidic mucin was determined using a computer-integrated microscope and an image analysis system (Leica QWin version 3.2.0; Leica Microsystems Imaging Solutions Ltd, Cambridge, UK). The slides were further used to determine the crypt area as previously described⁽Reference Hedemann, Eskildsen and Laerke²¹⁾.

Chemical analyses of diets

All feed samples were milled through a 0·5 mm mesh screen (Cyclotec 1093 Sample mill; Foss Tecator, Hoeganaes, Sweden) before analysis. The DM was determined by freeze-drying followed by drying at 105°C for 20 h, and ash was determined by combustion at 525°C for 6 h⁽²²⁾. Protein (N × 6·25) was determined as elementary N⁽Reference Hansen²³⁾. Starch⁽Reference Bach Knudsen²⁴⁾ and RS⁽Reference McCleary and Monaghan²⁵⁾ were determined by the enzymatic–colorimetric assays. Fructan was determined by an enzymatic–colorimetric method⁽Reference Larsson and Bengtsson²⁶⁾, modified as previously described⁽Reference Hindrichsen, Wettstein and Machmuller²⁷⁾. Neutral NSP and constituent sugars were analysed as alditol acetates by GC and uronic acids by colorimetry⁽Reference Bach Knudsen²⁴⁾. Klason lignin was measured gravimetrically as the residue resistant to 12 m-H₂SO₄ ⁽Reference Theander and Åman²⁸⁾.

SCFA in digesta

Digesta samples from the caecum and the colon were analysed for SCFA by GC⁽Reference Jensen, Cox and Jensen²⁹⁾.

Total RNA isolation

The caecum and the colon were opened lengthwise by a scissor and flushed with distilled water to remove the intestinal content. A small piece (approximately 5 mm) of tissue from the caecum and the colon was fixed overnight at 4°C in RNAlater (Sigma-Aldrich, Brøndby, Denmark), and then stored at − 80°C until analysis. Immediately before RNA extraction, the samples were thawed and approximately 15 mg of tissue was weighed and finely chopped with a scalpel. The samples were then homogenised in 350 μl of RNeasy lysis buffer and the homogenates were diluted with 70 % ethanol (1:1). The RNA was purified using the RNeasy mini kit (Qiagen, Albertslund, Denmark). The concentration and purity of RNA was assessed using NanoDrop ND-1000 spectrophotometer (NanoDrop Technologies, Inc., Wilmington, DE, USA).

Mucin mRNA analysis

The purified RNA was reverse transcribed with oligo-dT and random primers using superscript III RNase H-RT kit (Invitrogen, Taastrup, Denmark). The reverse-transcribed material (1 μl) was amplified with TaqMan Universal PCR Master Mix (Applied Biosystems, Stockholm, Sweden). The primers and probes were designed specifically for each gene by using Primer Express 2.0 software (Applied Biosystems). At least one oligonucleotide (primer or probe) was annealed to an exon boundary (exon structures reported for human subjects were used) to avoid the amplification of genomic DNA. The amplicon length was tested after the real-time RT-PCR analysis on a 2 % agarose gel and only one PCR product was amplified per gene, and the amplicon length agreed with the predicted length based on the nucleotide sequences (data not shown). The quantity of mRNA was detected by locked nucleic acid (LNA) fluorescent probes from the human library (https://qpcr2.probefinder.com/roche2.html) using an ABI 7900HT detection system (Applied Biosystems). The transcription of target genes were normalised according to hypoxanthine phosphoribosyltransferase (HPRT-1) transcription. Ideally, a housekeeping gene should not be regulated or affected by, for example, dietary factors, types of tissues, organs, sex, developmental and/or physiological stages, and it should be constitutively expressed. The expression of HPRT-1 was tested in isolated mucosa and muscle tissues from both the caecum and the colon, and the HPRT-1 expression was comparable in all four combinations of tissue and segment (caecal epithelium, caecal muscle, colonic epithelium and colonic muscle), thus supporting that HPRT-1 is a proper housekeeping gene in this experimental design. Furthermore, no dietary effect on the HPRT-1 expression was found when correcting for the loaded amount of total RNA.

The sequences of forward primers, LNA probes and reverse primers were as follows (accession numbers are given in parentheses):

• MUC-2 (U07615). 5′-GGGAACATGCAGAAGATCAACA-3′, 5′-TCCTGCTC-3′ (human LNA probe # 15), 5′-AGCCTCTCACATTCAGCTCGAT-3′

• MUC-3 (U76551). 5′-CCTCTGCTTGTCCACGGATACT-3′, 5′-GGTGGCAG-3′ (human LNA probe # 87), 5′-CGAGGATCACAAGAATCACCAA-3′

• HPRT-1 (NM_012583). 5′-GATTTTATCAGACTGAAGAGCTACTGTAATG-3′, 5′- TGGTGGAG-3′ (human LNA probe # 22), 5′-CCAGTGTCAATTATATCTTCAACAATCAA-3′

Statistical analyses

The thickness of the mucous layer was analysed using the mixed procedure (SAS Institute, Cary, NC, USA)⁽Reference Littell, Milliken and Stroup³⁰⁾ according to the following model:

where α_i is the effect of the diet (i = FF, C, R, I, RS or BH), U _j is the effect of the rat (j = 1, 2, …, 48), the effect of time, βt (t = 0, 15, 30, 45 and 60), was used as a covariate, β_it refers to the interaction between diet and time, and the term ɛ_ij~N(0,σ²) represents the random error. To account for the correlation between the intercept and the slope in the linear model, time was centred. The covariance structure was modulated using the option type = ar(1) to account for the correlation being higher for nearby times than far-apart times.

The morphological and histological data, and the concentration and proportions of SCFA, were analysed using the general linear model procedures (SAS Institute, Inc., Cary, NC, USA). The main effects of the diet and the block were assessed.

The mRNA quantities were analysed using the MIXED procedure (SAS Institute, Inc.)⁽Reference Littell, Milliken and Stroup³⁰⁾. The effects of the NDC source were tested in a model including the block as a fixed effect and the weight at slaughter as a covariate to account for the differences in body mass. All statistics were performed at the ΔCt stage (Ct of the target gene − Ct of HPRT-1)⁽Reference Theil, Sorensen and Therkildsen³¹⁾. The relative mRNA quantity was calculated by using the formula: Relative mRNA quantity = 2^− ΔΔCt.

Pearson's correlations were used to evaluate the relationship between the total thickness of the mucous layer and the area of mucin in the colon or the concentration and proportion of SCFA in digesta based on the measurements obtained from individual rats (n 48; Table 5). Furthermore, Pearson's correlations between the MUC2/MUC3 transcriptions and SCFA production were tested based on the mean levels within a dietary treatment (n 6; Table 6) to evaluate whether specific SCFA in the caecum or the colon affected the mRNA abundance in the respective tissues. Similarly, the correlations between the MUC2/MUC3 transcriptions and thickness of the mucous layer in the colon were tested to evaluate whether altered transcription of the studied genes was responsible for the observed differences in the total mucous layer.

Table 5 Correlations between the thickness of the total mucous layer after 60 min and the mucin-staining area, the abundance of MUC genes, and the concentration and proportion of SCFA in digesta in the colon

(Correlation coefficients and P values)

Table 6 Correlations between the abundance of MUC2 and MUC3 mRNA and the mean SCFA pools and the mean proportions of SCFA in the caecum and the colon

(Correlation coefficients and P values)

The results on morphology, mucin-staining area and SCFA are expressed as least-squares means with their pooled standard errors. For the total mucous layer, the adherent mucous layer and the expression of MUC2 and MUC3, the mean values are presented. Treatment differences are considered to be significant at α = 0·05.