Bacterial strains and culture

ETEC (serotype O149:K91: K88ac) was obtained from the China Institute of Veterinary Drugs Control (Beijing, China). Luria-Bertani (LB) and LB agar broth were prepared (yeast extract, 0·5 g; NaCl, 1 g; peptone, 1 g; double-distilled water, 50 ml; agar powder, 2 % for LB agar broth) and sterilised under 121°C, 0·11 MPa for 20 min (pH = 6). The bacteria were resuscitated in 3 ml of LB broth at 37°C for 24 h with shaking and plated onto LB agar. A single colony was inoculated into 50 ml of LB broth, cultured overnight at 37°C and 250 rpm and then subcultured and serially diluted on LB agar for bacterial enumeration^{(Reference Gao, Han and Huang21)}.

Animal diets and experimental design

A total of thirty-two male Duroc × Landrace × Yorkshire pigs weaned at 21 d (with an average body weight of 6·48 (se 0·14) kg) were randomly allotted into a 2 (MOS) × 2 (ETEC) factorial experiment of four treatments composed of CON (pigs were fed with a basal diet), CMOS (pigs were fed with basal diet containing 3 g/kg MOS product), ECON (pigs were fed with a basal diet and challenged by ETEC) and EMOS (pigs were fed with basal diet containing 3 g/kg MOS product and challenged by ETEC). As the purity of the MOS product is 20 %, the final concentration of the pure MOS in the diet is 0·6 g/kg. The number of pigs used in each group (n 8) meets this minimal requirement of statistic for digestible trials or mechanism studies (e.g. six replicates are acceptable)^{(Reference Gao, Han and Huang21,Reference Agazzi, Perricone and Zorini22)} . Pigs received the same parental nutrition and management (e.g. sows were fed with the same diet, synchronisation estrous). The trial lasted for 21 d. On 19th day, the challenge groups were orally treated with 100 ml of LB culture containing 1 × 10¹⁰ colony-forming units/ml of ETEC by using an orogastric tube lasted for 3 d, whereas the non-challenge groups were orally treated with equivalent amount of culture medium^{(Reference Liu, Piao and Thacker23)}. The basal diet (Table 1) was formulated to meet the swine nutrient requirements recommended by the National Research Council⁽²⁴⁾. Pigs were individually housed in 1·5 × 0·7 m² metabolism cage and were given ad libitum access to feed and fresh water with the room temperature controlled between 25 and 28°C, relative humidity 65 % (se 5) %.

Table 1. Experiment basal diet composition and nutrient level

* The vitamin premix provided the following per kg of diet: 2·7 mg of vitamin A, 75 μg of vitamin D₃, 20 mg of vitamin E, 3 mg of vitamin K₃, 1·5 mg of vitamin B₁, 4 mg of vitamin B₂, 3 mg of vitamin B₆, 0·02 mg of vitamin B₁₂, 30 mg of niacin, 15 mg of pantothenic acid, 0·75 mg of folic acid and 0·1 mg of biotin.

† The mineral premix provided the following per kg of diet: 100 mg Fe, 6 mg Cu, 100 mg Zn, 4 mg Mn, 0·30 mg iodine, 0·3 mg Se. The diet was formulated based on the recommendation of the National Research Council⁽²⁴⁾.

Sample collection

Feed samples were collected at the beginning of the experiment and stored at −20°C for nutrient analysis, during days 14–17 of the experiment; fresh faecal samples were collected immediately after excretion from pigs in each cage, weighed and added 10 ml 10 % H₂SO₄ solution to per 100 g of fresh faecal. The feed and faecal samples were dried at 65°C for 2 d, ground to pass through a 1-mesh screen and then stored at −20°C until measurement for nutrients digestibility. Blood samples were obtained on day 22 by jugular vein puncture and placed in two 10-ml vacuum tubes. One tube for blood parameters was analysed, and the serum was collected after centrifugation of another tube at 3500 g and stored at –20°C until the serum indexes analysis. At the end of the trial, pigs were anaesthetised by intravenous injection with sodium pentobarbital (200 mg/kg body weight) and the tissues of the duodenum, jejunum and ileum were immediately isolated. At the same time, the duodenal, jejunal and ileal middle segments (4 cm obtained from the middle of each intestine) were gently flushed with ice-cold PBS, followed by fixation in 4 % paraformaldehyde solution for morphological analyses. Besides, digesta from caecum was collected, and the intestinal mucosa was obtained from the residual intestinal segments with a scalpel blade and placed in frozen tube and then frozen by immersion in liquid N₂ and stored at −80°C until analysis.

Growth performance evaluation

All pigs were weighed before feeding on days 1, 19 and 22. Feed intake and waste feed were recorded every day throughout the experiment which could be provided to calculate the average daily feed intake, average daily gain and the feed:gain ratio (the type of scale used in this study is electronic scale; 0–1, 0–20 kg, respectively).

Apparent total tract nutrient digestibility analysis

The frozen dried and milled feed and faecal samples were used for nutrient digestibility analysis, which uses acid insoluble ash as endogenous indicators, a method described by the Chinese National Standard (GB/T23742-2009). The DM, crude protein, ether extract and ash contents were determined according to AOAC⁽²⁵⁾, whereas the gross energy content was measured by an adiabatic bomb calorimeter (LECO) to calculate the apparent total tract digestibility. All contents were calculated by the following formula: (100 − A1F2/A2F1 × 100)^{(Reference Yang, Iji and Kocher26)}. A1: digesta nutrient; A2: digesta acid insoluble ash; F1: diet acid insoluble ash; F2: digesta acid insoluble ash.

Serum pro-inflammatory cytokines and Ig detection

The concentration of pro-inflammatory cytokines (TNF-α, IL-1β and IL-6)and Ig (IgG, IgM and IgA) in serum was determined by following the instructions of a commercially available porcine ELISA kits (Jiangsu Jingmei Biotechnology Co. Ltd). All procedures were guided by manuals of the kits. For quantification, the standards provided in the kits were used to generate standard curves.

Histomorphology analysis of each intestinal segment

The fixed intestinal segments were dehydrated through a graded series of ethanol and then embedded in paraffin^{(Reference Wan, Zhang and Chen27)}. Cross sections of each sample were prepared, stained with haematoxylin–eosin (H&E) and then sealed with neutral resin. Finally, ultrathin sections of the duodenal, jejunal and ileal samples were examined for crypt depth and villus height with image processing and analysis system (Image-Pro Plus 6.0). The method of measurement of crypt depth and villus height was followed by King’s and Wan’s. A total of ten intact, well-oriented, crypt-villus units were analysed in triplicate per intestinal segment^{(Reference Wan, Zhang and Chen27,Reference King, Morel and Revell28)} . The ratio of villus height:crypt depth (V:C) was calculated from the data described above.

Enzyme activity

The frozen duodenal, jejunal and ileal mucosa were homogenated in chilled saline at a ratio of 1:9 (w/v) for 15 min. The homogenate was centrifuged at 3500 g for 10 min at 4°C, and the supernatant was used in spectrophotometric assays for protein content, which was used to calculate the alkaline phosphatase and digestive enzymes (lactase, sucrase and maltase) activity following the instructions described by commercial kits (Jiancheng Bioengineering Ltd). Enzyme activity was defined as hydrolysis of 1 mol of the substrate per mg of protein tissue per minute under the condition of 37°C, pH = 6·0.

Caecal microbiological analysis

Approximately 200 mg caecal digesta was weighed and treated using the Stool DNA Kits (Omega Bio-Tek) following the manufacturer’s instruction to extract total DNA for quantification real-time PCR, which was performed by conventional PCR on the Opticon DNA Engine (Bio-Rad). Total bacteria were detected by the reaction which runs in a volume of 25 μl with 1 μl of forward and 1 μl of reverse primers (100 nm), 12·5 μl SYBR Premix Ex Taq (2 × concentrated), 2 μl template DNA, 1 μl 50 × ROX Reference Dye*3 and 7·5 μl of RNase-Free ddH₂O. The SuperReal PreMix (Probe) kit (Tiangen Biotech Co. Ltd) was used for Lactobacillus, E. coli, Bacillus and Bifidobacterium detection, and primers and fluorescent oligonucleotide probes are presented in online Supplementary Table S1. Each reaction was run in a volume of 25 μl with 12·5 μl 2 × Super Real PreMix (Probe), 1 μl of forward and 1 μl of reverse primers (100 nm), 1 μl 50 × ROX Reference Dye*3, 1 μl probe (100 nm), 2 μl DNA and 6·5 μl of RNase-Free ddH₂O. All reaction protocols were composed of one cycle of pre-denaturation at 95°C for 15 min; forty cycles of denaturation at 95°C for 3 s; annealing and extension at 60°C for 30 s. The cycle threshold values and baseline settings were determined by automatic analysis settings, and the copy numbers of the target group for each reaction were calculated from the standard curves, which were generated by constructing standard plasmids by a 10-fold serial dilution of plasmid DNA (1 × 10¹ to 1 × 10⁹ copies/μl).

Isolation and reverse transcription of RNA from intestinal mucosa and quantitative PCR

The frozen duodenal, jejunal and ileal mucosa samples (about 0·1 g) were ground in liquid N₂ and homogenised in 1 ml of RNAiso Plus (Takara Biotechnology Co. Ltd) to extract total RNA followed the manufacturer’s instructions, and the purity and concentration of total RNA were detected by using a spectrophotometer (NanoDrop 2000, Thermo Fisher Scientific, Inc.); samples which OD260:OD280 ratio ranged from 1·8 to 2·0 were deemed appropriate. Subsequently, a volume equivalent to 1 μg total RNA from each duodenal, jejunal and ileal sample was used for reverse transcription into cDNA, which was based on the protocol of PrimeScript™ RT reagent kit with gDNA Eraser (Takara Biotechnology Co. Ltd). This process consists of two steps: I: 37°C for 15 min, II: 85°C for 5 s.

The expression level of the target gene in intestinal mucosa was quantified using quantitative PCR, the oligonucleotide primer sequences used in quantitative PCR are presented in online Supplementary Table S1 and quantitative PCR was performed with the SYBR® Green PCR I PCR reagents (Takara Bio Inc.) using a CFX96 Real-Time PCR Detection System (Bio-Rad Laboratories). All cDNA samples were detected in triplicate. The reaction mixture (10 μl) contained 5 μl SYBR Premix Ex Taq II (Tli RNaseH Plus), 0·5 μl forward primer, 0·5 μl reverse primer, 1 μl cDNA and 3 μl RNase-Free water. The protocol used in quantitative PCR was as follows: 95°C for 30 s, followed by 40 cycles: at 95°C for 5 s and 60°C for 34 s. The generated gene-specific amplification products were confirmed by melting curve analysis after each real-time quantitative PCR assay. The housekeeping gene β-actin was used to standardise the mRNA expression level of target genes, which was calculated based on the 2^–ΔΔCt method^{(Reference Fleige, Walf and Huch29)}.

Sample size calculation and statistical analysis

The minimal sample size was calculated based on the experimental design (repeated-measures, between-factors ANOVA) determining the MOS × ETEC effect to the intestinal health as the primary outcome measure. We used G*Power software (version 3.1.9.2) for the power analysis with following variables; the power = 0·8, significant level = 0·05 and effect size = 0·35 in the experiment. The effect size was estimated based on the results from a preliminary study. Hence, the required minimal sample size was five pigs per group.

The data collected before the ETEC challenge were analysed by one-way ANOVA. After the challenge, the data were analysed by two-way ANOVA with the General Linear Model procedure of SPSS as a 2 (MOS) × 2 (ETEC) factorial design. P value < 0·05 was deemed to be significant and the P value between 0·05 and 0·1 to show a significant trend. Duncan’s multiple range test was used based on the ANOVA, which showed a significant difference. All data were analysed by SPSS 24.0 (SPSS, Inc.) and expressed as means with their standard errors.