Ethics statement

The trial was approved by the Animal Care and Use Committee of China Agricultural University (approval number 20130611–1).

Experimental design

Eight Simmental bulls (initial body weight 219 (sd 14) kg, 10 months old) castrated 2 weeks before the trial started were used as the experimental animals. The RSC used in the trial was the rapeseed residue after the oil was extracted by hot pressing at the temperature of 120°C with the pressure of approximately 20 MPa for 20 min/50 kg rapeseed. Four levels of hot-pressed RSC, that is, 0·00, 2·65, 5·35 and 8·00 % DM, were included in the rations as the experimental treatments (Table 1). The animals and the experimental treatments were randomly assigned in a replicate 4 × 4 Latin square design. Each animal was supplied with 3·5 kg DM of total mixed ration daily, which was approximately 90 % of the ad libitum DM intake measured in a preliminary trial. The concentrations of CP and net energy of the rations were 1·2 times the maintenance requirements for the steers^{(Reference Feng19)}. Each experimental period lasted 20 d, including 15 d for adaptation and 5 d for sampling. The animals ate all the feeds offered daily, and no feeds were left during the trial.

Table 1. Ingredients and nutritional composition of experimental rations (% DM)

(Percentages)

RSC, rapeseed cake; NEmf, net energy for maintenance and fattening of beef cattle; CP, crude protein; RDP, rumen degradable protein; RUP, rumen undegradable protein.

* Provided per kg DM of ration: 54 mg Zn (ZnSO₄); 70 mg Fe (FeSO₄); 38 mg Mn (MnSO₄); 12·8 mg Cu (CuSO₄); 1·2 mg iodine (KI); 0·17 mg Se (Na₂SeO₃); 0·6 mg Co (CoCl₂); 2·31 mg vitamin A; 75 µg vitamin D₃.

† NEmf was calculated according to Feng^{(Reference Feng19)}.

‡ The contents of RDP and RUP were determined according to Licitra et al.^{(Reference Licitra, Hernandez and Van Soest22)} and the National Research Council⁽²³⁾.

Animal feeding and sampling

The animals were kept in individual pens. The daily ration was divided into two equal meals that were given at 07.00 and 16.00 hours. Fresh drinking water was freely available. During the sampling period, the total faeces from each animal was collected using a plastic bucket and the weight of the faeces was recorded daily. An amount of 2 % of the total faeces from each animal was sampled after homogenisation and mixed with sulphuric acid (concentration 10 %, v/v) at 20 ml/100 g fresh faecal sample to keep the pH of the samples below 3·0 and prevent N loss during storage and analysis. The ruminal fluid was taken through the oesophagus of each animal using a tube 2 h after feeding in the morning on the third day of each sampling period. To avoid saliva contamination, the first sample of rumen fluid was discharged and then a sample of about 200 ml of rumen fluid was collected from each steer. The rumen fluid was filtered through four layers of cheesecloth, and the ruminal pH was immediately measured using a portable pH meter (model 8601, AZ Instrument Corp. Ltd). The feeds were also sampled daily. The samples were stored in a freezer at –20°C until later analysis within 2 months.

Chemical analysis of feeds and faeces

The samples of feeds and faeces were freeze-dried (LGJ-12, Beijing Songyuan Huaxin Technology Development Co. Ltd) and then grinded to pass a sieve with the pore size of 1 mm for determination and analysis. The DM of feeds and faeces was determined in an oven at 105°C using the no. 934.01 AOAC method (1998)⁽²⁰⁾. The crude ash of the feeds and faeces was determined by combustion in a muffle furnace at 550°C, and the total N of feeds and faeces was analysed by the Kjeldahl method according to AOAC methods (1998)⁽²⁰⁾ no. 942.05 and 988.05, respectively. The organic matter of the feeds and faeces was calculated by DM minus crude ash. The ether extract (EE) of the feeds and faeces was analysed according to AOAC (1998)⁽²⁰⁾ method no. 920.39. The neutral-detergent fibre and acid-detergent fibre of the feeds and faeces inclusive of residual ash were analysed on an Ankom A200i Fiber Analyzer (Ankom Technology Corp.) using the methods of Van Soest et al.^{(Reference Van Soest, Robertson and Lewis21)}. The rumen degradable protein and rumen undegradable protein contents of the feeds were calculated based on Licitra et al.^{(Reference Licitra, Hernandez and Van Soest22)} and the National Research Council⁽²³⁾. The extraction of GLS from RSC was conducted according to Tholen et al.^{(Reference Tholen, Shen and Truscott24)}, and the content of GLS in RSC was analysed using the method of Wathelet et al.^{(Reference Wathelet, Wagstaffe and Biston25)} with slight modification.

Rumen fermentation parameters

The ammonia nitrogen (NH₃-N) concentration of rumen fluid was determined using the colorimetric method of Broderick & Kang^{(Reference Broderick and Kang26)}. The volatile fatty acid (VFA) concentration of rumen fluid was determined via a GC (TP-2060F, Beijing Beifen-Ruili Analytical Instrument Co. Ltd) using the method described by Yang et al.^{(Reference Yang, Wei and Zhao27)}. The ruminal concentration of SCN was analysed according to China Hygiene Standard WS/T 39-1996⁽²⁸⁾. The ruminal concentration of ISCN was analysed using the method of Matthäus & Fiebig^{(Reference Matthäus and Fiebig29)}. The ruminal concentration of goitrin was analysed using the method of Thomke et al.^{(Reference Thomke, Pettersson and Neil30)}.

Real-time quantitative PCR analysis for ruminal microflora

The genomic DNA of the ruminal micro-organisms was extracted using the TIANamp Stool DNA Kit (DP328, Tiangen Biotech Co. Ltd). The primer sequences for the target species (Table 2) of ruminal microflora were synthesised by Sangon Biotech Co. Ltd. The real-time PCR was performed with TB Green^TM Premix Ex Taq^TM (Tli RNaseH Plus) from Takara Biomedical Technology Co. Ltd. (no. RR420A) on a Funglyn FTC-3000 Real-time PCR System to determine the relative abundance of the target species using the protocol described by Yang et al.^{(Reference Yang, Wei and Zhao27)}. The abundance of the microbial 16S rDNA gene copy number was expressed relative to the copy number of the total rumen bacterial 16S rDNA using the following equation:

Table 2. Real-time PCR primers of ruminal microbial flora

* Primer direction (F: forward; R: reverse).

$${\rm{Relative\;abundance\;of\;target\;}}\left( {\rm{\% }} \right){\rm{\;}} = {2^{ - \left( {{\rm{Ct\;target}} - {\rm{Ct\;total\;bacteria}}} \right)}} \hskip 170pt\times 100$$

,

where Ct represents the threshold cycle.

Sequencing of rumen bacterial 16S rRNA gene

The total genomic DNA from the ruminal fluid samples for 16S rRNA gene sequencing was extracted using the CTAB/SDS method. The targets in the V3-V4 region of the bacterial 16S rRNA gene were amplified using 341F (5′-CCTAYGGGRBGCASCAG-3′) and 806 R (5′-GGACTACHVGGGTWTCTAAT-3′)^{(Reference Frank, Rogers and Olins36)}. All PCR were carried out in 30 μl reactions with 15 μl of Phusion® High-Fidelity PCR Master Mix (New England Biolabs), 0·2 μm of forward and reverse primers, and approximately 10 ng of template DNA. The PCR thermal cycling was carried out as follows: 98°C for 1 min (one cycle); 98°C for 10 s, 50°C for 30 s, and 72°C for 30 s (thirty cycles); and finally 72°C for 5 min. The amplicons were sequenced on an Ion S5^TM XL platform (Thermo Fisher Scientific), and 400 bp/600 bp single-end reads were generated.

Metagenomic analysis of ruminal bacterial community

Following sequencing, raw 16S rRNA gene sequencing reads were subjected to quality filtration according to the Cutadapt (version 1.9.1)^{(Reference Martin37)} quality-controlled process and compared with the Silva database^{(Reference Quast, Pruesse and Yilmaz38)}. The taxonomic analysis of representative operational taxonomic unit (OTU) sequences with ≥97 % similarity was analysed using UPARSE software (version 7.0.1001)^{(Reference Edgar39)}. For each representative sequence, the Silva database was used to annotate the taxonomic information based on the Mothur algorithm^{(Reference Quast, Pruesse and Yilmaz38)}. The bacterial richness values including Chao1, abundance-based coverage estimator, community diversity (Shannon and Simpson index) and sequencing depth (Good’s coverage) were calculated using QIIME (version 1.7.0)^{(Reference Caporaso, Kuczynski and Stombaugh40)}. The Phylogenetic Investigation of Communities by Reconstruction of Unobserved States was used to predict the metabolic functions of the microbial communities based on the bacterial OTU^{(Reference Langille, Zaneveld and Caporaso41)} in combination with the Kyoto Encyclopedia of Genes and Genomes software^{(Reference Kanehisa and Goto42)}.

Statistical analysis

Statistical analysis was performed using a linear regression model with cluster robust standard errors clustered on steers in Stata (version 15, StataCorp 2017). The model for statistical analysis including fixed effects of RSC ration (x ₁ = 0, 1, 2 and 3), period (x ₂ = 1, 2, 3 and 4) and standard errors was adjusted for clusters of steers (n 8) for the variables. The statistical analysis results were presented as the intercept of the regression equation, regression coefficients, robust se and CI for RSC ration. The P values for regressions were also presented. The data were declared to be significant at P < 0·05 and as tendencies at 0·05 < P < 0·10. Spearman’s rank correlation tests between bacterial species at the genus level and the environmental factors including pH and the ruminal concentrations of NH₃-N, total VFA and SCN were performed, and the significance was tested by corr.test in the psych package from R software (version 2.15.3, R Core Team 2013, http://www.r-project.org).