Care and use of animals

All handling practices followed the recommendations of Directive 2010/63/EU of the European Parliament, the Council on Protecting Animals used for scientific purposes, and the IGM-CSIC Animal Experimentation Committee (protocol 736/2018). The study reported in the manuscript follows the recommendations in the ARRIVE guidelines. ^{Reference Percie du Sert, Hurst and Ahluwalia15}

Animals, diets and feed efficiency measurement

CSIC conducted feeding trials using 16 female dairy calves born in the same commercial farm and selected to minimise the range of live body weight (LBW) and day of birth. These animals were separated from the cows in the first 24 hours of life and fed 3 L of colostrum daily until day 3 of life. Starting at 3 days, once housed in individual straw-bedded hutches, they were allocated to one of two groups (n = 8 per group; control and EO) balanced according to the body weight at birth. Calves were fed MR (145 g of Novilac Turbostart, Schils/L) twice a day using a bucket with a nipple (allowing the reflex closure of the oesophageal groove) until day 45. During this phase, these animals were fed daily a fixed amount of reconstituted MR (divided into two feedings, at 09:00 a.m. and 6:00 p.m.) that was gradually increased from 3 to 7 L at the same rate for all the individuals.

Moreover, the animals in the EO group were supplied daily with 0.23 ml of oregano EO, accounting for 200 mg of carvacrol (Zane Hellas 100%) diluted in the first 100 mL of MR for 45 days. No concentrates were offered, and no leftovers of MR remained during this phase, so dry matter intake was similar for all calves. All the animals were weighed at birth and on days 4, 10, 25 and 45 of life (e.g., at the end of the EO administration period) to estimate the average daily gain (ADG) and then calculate the feed-to-gain conversion rate during the suckling period.

Animals were managed in a feedlot once they reached 45 days of age using an automatic feeding machine until weaning (70 days of life) programmed to control the total amount of MR (without EO) consumed by each animal [recognised by radio frequency identification (RFID) ear tags]. Thus, the automatic feeding systems stopped delivering MR when each animal had reached a total accumulated dry matter intake of 54 kg MR. During this phase, animals were allowed access to a starter feed compound (ad libitum).

After weaning (70 days of life), all the calves were managed in the feedlot and fed with a total mixed ration (TMR-1; Barley straw, 120 g/kg; dehydrated alfalfa, 140 g/kg; concentrate, 740 g/kg) formulated (with no EO) to cover their nutritional requirements during the first post-weaning period (up to 6 months of life) and a second TMR (TMR-2, with no EO) with a higher amount of fibre during the replacement phase (6-12 months of life). Voluntary feed intake was recorded individually daily using control feed intake devices (Agrolaval S.L., Gijón, Asturias, Spain) and RFID ear tags for 70 days, starting when animals were, on average, 322 days old. Daily sampling of TMR-2 after mixing (before feeding) and sufficient mixing and subsampling to minimise sampling error was conducted. Weekly analysis of daily composited feed samples of TMR-2 supplied to dairy cows was performed for DM (ISO 6496:1999), ash (ISO 5984:2002), CP (ISO 5983:2009), amylase-treated neutral detergent fibre [(aNDF), NDF assayed with a heat-stable amylase and expressed inclusive of residual ash; Ankom Technology Corp., Macedon, NY, USA] and ADF (ADF expressed inclusive of residual ash; Ankom Technology Corp., Macedon, NY, USA). The ingredients and chemical composition of TMR-2 administered during the feed intake control period are summarised in Table 1.

Table 1. Ingredients and chemical composition (g/kg DM unless otherwise stated) of the total mixed ration (TMR-2) consumed by the heifers during the replacement phase

^a Amylase-treated neutral detergent fibre.

Animals were weighed monthly during the replacement phase to measure feed efficiency traits regarding the feed-to-gain ratio and residual feed intake (RFI). Average daily weight gain (ADG, g/d) was estimated as the regression coefficient (slope) of LBW against time using the REG procedure of the SAS package (SAS Institute Inc., Cary, NC). The feed-to-gain ratio was obtained by dividing daily feed intake by the ADG (g/d). RFI was calculated using a multiple linear regression model. The DMI, ADG and mid-test metabolic body weight data (MBW, as LBW^0.75) of all the calves were introduced. The statistical model used was Y_i = β ₀ + β ₁ MBW_i + β ₂ ADG_i + e_i , where Y_i represents the predicted feed intake of the i _th animal; β ₀ is the equation intercept; β ₁, the regression coefficient on MBW; β ₂, the regression coefficient on ADG and e_i , the residual of the i_th animal. Thus, this prediction may be considered the ‘average’ or expected value for animals of similar weights and rates of gain. The actual daily feed intake minus the predicted feed intake of each individual corresponds to the RFI, so the RFI value is inversely related to the feed efficiency.

Blood and faecal sampling

Three blood sampling times, 3 (T0), 45 (T1) days and 13 months old (T2), were planned. Blood samples were collected into glass tubes by venipuncture (tail or jugular). Tubes with no anti-coagulant were allowed to clot at room temperature and then centrifuged at 3.520 × g for 16 min at 4 °C. After that, the obtained serum samples were stored at –80 °C until use in biochemical profiling. A second blood sample was collected into tubes containing lithium-heparin, placed in iced water and centrifuged at 3.520 × g for 16 min at 4 °C. Then, plasma samples were stored at –80 °C until use in metabolomics. As explained below, a third blood sample collected into a lithium-heparin tube was used for flow cytometry analyses to measure several peripheral blood mononuclear cells (PBMCs) markers such as CD4⁺, CD8⁺, CD21⁺, WC1⁺ and CD14⁺.

Two sampling times for faeces [45 days (T1) and 13 months old (T2)] were planned. Faecal samples (rectal grab samples) were collected before the morning meal and stored at −80 °C until freeze-drying and use in either total apparent digestibility (T2) determination according to Keulen and Young (1997) ^{Reference Van Keulen and Young16} or total DNA (T1 and T2) extraction as explained below.

Biochemical profile and antioxidant status

Serum samples were stored at –80 °C until used for the analysis of the biochemical profile (albumin, aspartate aminotransferase [AST/GOT], gamma-glutamyl transpeptidase [GGT], beta-hydroxybutyrate [BHB], total bilirubin, Ca, Zn, Mg, ceruloplasmin, creatine kinase, creatinine, high-density lipoprotein [HDL], low-density lipoprotein [LDL], cholesterol, glucose, insulin, non-esterified fatty acids [NEFA], triglycerides, urea, protein and globulin). The biochemical profile was measured using clinical chemistry and the turbidimetry analyser Biosystems BA400 (Biosystems S.A., Barcelona, Spain). According to the manufacturer’s instructions, superoxide dismutase activity (SOD) was assayed using a Sigma Aldrich kit (Ref. 19160).

Flow cytometry analyses on the mononuclear cell population

PBMCs were isolated from 30 mL of heparinised blood by density-gradient centrifugation with Lymphoprep^™ (STEMCELL Technologies Cologne, Germany) as previously described elsewhere. ^{Reference Arteche-Villasol, Benavides and Espinosa17} The resultant PBMCs were washed three times with PBS, pelleted and resuspended in supplemented RPMI1640 medium + GlutaMAX^™ with phenol red (Gibco, Paisley, UK). PBMCs were counted in a Neubauer chamber and adjusted to a final concentration of 10⁶ cells mL⁻¹. Cell viability (> 90%) was assessed by Trypan blue dye exclusion.

Single-colour flow cytometry analyses were performed as previously described. ^{Reference Arteche-Villasol, Gutiérrez-Expósito and Vallejo18} Briefly, a total of 2 × 10⁵ cells per well were seeded in different wells in a 96-well plate (Thermo Fisher Scientific, Roskilde, Denmark) and individually incubated with non-conjugated anti-bovine CD4 (MCA834GA, Bio-Rad®), CD8 (MCA837GA, Bio-Rad®) and CD21 (MCA1424GA, Bio-Rad®) as primary antibodies at a 1:400 dilution for 1 h at 4 °C. Cells were washed twice with PBS and incubated with fluorescein isothiocyanate (FITC)-conjugated anti-mouse IgG (F0313, Dako®) as a secondary antibody at a dilution of 1:50 for 1 h at 4 °C in the dark. At the same time, cells from two wells were also individually incubated with FITC-conjugated anti-bovine CD14 (MCA2678F, Bio-Rad®) and WC1 (MCA383F, Bio-Rad®) antibodies at a 1:400 dilution for 1 h in the darkness at 4 °C. Finally, the wells were washed twice with PBS, and the cells were fixed with 1% CellFIX^™ (Becton Dickinson and Company, Erembodegem, Belgium) and kept in the dark until flow cytometric analysis.

Sample acquisition and data analysis were performed as previously described by Arteche-Villasol et al. (2020). ^{Reference Arteche-Villasol, Benavides and Espinosa17} At least 10,000 events were acquired using a MACSQuant flow cytometer (Miltenyi Biotec®) and gated to discard the presence of air and doublets. Then, the data were analysed using MACSQuantify10 Software^™ (Miltenyi Biotec®), and the results were expressed as a percentage of positive cells for each lymphocyte surface marker.

Microbiota characterisation of faecal samples

DNA was extracted from each faecal sample using a QIAamp Fast DNA Stool Mini Kit (Qiagen, Germany), according to the manufacturer’s protocol. DNA quality and quantity were assessed using a NanoDrop ND-1000 spectrophotometer (NanoDrop Technologies, Wilmington, DE, USA). The isolated DNA was then stored at −20 °C until use. Then, bacterial DNA was amplified using primers to target the V3–V4 hypervariable regions of the 16S rRNA gene, as previously described. ^{Reference Caporaso, Lauber and Walters19} DNA Sequencing, bioinformatic processing and statistical analysis were performed as described in Ranilla et al. (2023). ^{Reference Ranilla, Andrés and Gini20}

Metabolomics analysis

A volume of 400 µL of ice-cold methanol (LC-MS grade) was added to 100 µL of plasma sample containing 5 µL of internal standard (15N L-Leucine, 98%, Sigma –Aldrich, 1 mg/mL), vigorously vortexed and then stored for 30 min at − 20°C. Samples were centrifuged at 14,800 r.p.m. for 10 min at + 4°C. The supernatant was transferred to a new tube and dried under a stream of nitrogen. The residue was reconstituted in 100 µL of mobile phase (1% of 0.1% formic acid in acetonitrile – FM B) and analysed by LC-QTOF-MS. A blank sample (100 µL of water LC-MS grade) and a quality control sample (QC, a pool of all samples analysed) were also prepared.

Five microlitres of each sample were injected in duplicate. The autosampler and column temperatures were set at 10°C and 40°C, respectively. The analytes were eluted using a CORTECS UPLC T3 C18 (2.1 × 150 mm, 1.6 µm) (Waters™) connected to an ExionLC™ AD system (Sciex™) using 0.1% formic acid in water as mobile phase A and 0.1% formic acid in acetonitrile as mobile phase B. The gradient was from 99% A to 5% A in 8 min, with a total run of 20 min at a flow rate of 0.4 mL/min. The separated metabolites were then ionised using a Turbo V™ Ion Source with an ESI Probe source (Sciex™) and analysed in a ZenoTOF 7600 System equipped with a Zeno trap (Sciex™). Mass spectra were collected, in both positive- and negative ion modes, in Full-Mass Scan from 50 to 1500Da (250 ms accumulation time) and in IDA® mode (Information Dependent Acquisition) from 40 to 1500Da (50 ms accumulation time). For both methods, ion source gas 1 (GS1) and 2 (GS2) were set to 40 and 55 psi, respectively; the curtain gas to 25 psi, CAD gas to 7 and the source temperature to 550°C. The Spray Voltage was fixed at 4.5 kV (−4.5 kV in negative mode), the declustering potential (DP) was 80 eV and the collision energy was 30 eV with a collision energy spread of 15 eV.

The data were analysed using SCIEX OS 2.2 software (SCIEX™), in two processing functions: (1) FormulaFinder, to identify possible compound formulas based on TOF-MS spectra (compound molecular weight); (2) LibraryView™ (ver 1.0) to search MS/MS spectra with the built-in accurate mass spectral library (Metabolite High-Resolution MS/MS Spectral Library). Data were expressed as the ratio of the analytes versus the internal standard. The average corresponding area’ was normalised to the estimated protein concentration in each extracted sample. Identifications (ID) were obtained based on the value m/z (parent ion) achieved and determined in high resolution.

Statistical analyses

Feed efficiency traits and digestibility were analysed by one-way ANOVA, whereas the biochemical profile, SOD and PBMCs were assessed by repeated measurements using the MIXED procedure of SAS. In the repeated measurement analysis, data from the first sampling day (day 3, before including EO in the MR of the EO group) was used as a covariate, and adjusted mean values were estimated when the effect was significant.

Regarding the faecal microbiota, differences between groups (EO vs. control) along time points in terms of OTU abundances and diversity indices were evaluated with the three following linear models: linear model A: Y_ik = μ + timepoint_k + e_ik, or linear model B: Y_ij = μ + treatment_j + e_ij, or linear model C: Y_ikj = μ + timepoint_k + treatment_j + e_ikj, where Y_kj is the abundance (counts) or index value for each taxonomy (OTU) and diversity metric per sample _i in timepoint _k and treatment _j; timepoint_k is the effect of the categorical variable time point (2 classes); treatment_j is the effect of the categorical variable treatment (2 classes); e_kj are the residuals of the model. Faecal microbial diversity was assessed within- (alpha-diversity) and across- (beta-diversity) samples. All indices (alpha- and beta-diversity, previously listed in Ranilla et al. 2023) ^{Reference Ranilla, Andrés and Gini20} were estimated from the complete OTU table and filtered for OTUs with more than 10 total counts distributed in at least two samples. Details about the indices used can be found in Appendix S2 of Biscarini et al. (2018). ^{Reference Biscarini, Palazzo and Castellani21} Beta-diversity significances were tested using PERMANOVA.

MetaboAnalyst 5.0 ^{Reference Pang, Chong and Zhou22} was used to perform multivariate data analyses, including principal component analysis (PCA), Partial Least Squares Discriminant Analysis (PLS-DA), heat maps, hierarchical clustering and pathway analysis ^{Reference Pang, Chong and Zhou22} Volcano plots were drawn at T0 (3 days), T1 (45 days) and T2 (13 months) to identify significant metabolites between treatments. Plots used a threshold of 1.5 for fold change (FC) on the × axis and a threshold of 0.05 for the false-discovery rate (adjusted P-value) on the y axis.