Ethical approval

Protocols were developed in accordance with the Cruelty to Animals Act (Ireland 1876, as amended by European Communities regulations 2002 and 2005) and the European Community Directive 86/609/EC. In Ireland, the study was approved by the Teagasc Animal Ethics Committee (TAEC145/2017) and all animal procedures performed were conducted under experimental license from the Health Products Regulatory Authority (AE19132/P065). In Norway, the study was approved by Norwegian Food Safety Authority (FOTS ID 13168). In France, the study was approved by the ethics committee and the Ministry of Research.

Experimental design

The aim of this experiment was to characterize the sialic acid species of the cervical mucins in six ewe breeds with known differences in pregnancy rates following cervical AI using frozen–thawed semen. This study was part of larger project that aimed to interrogate the ewe breed differences in cervical mucus properties and anatomical characteristics across the estrus cycle of both synchronized (using progestogen pessaries combined with equine chorionic gonadotropin) and natural cycles. A description of the experimental model, animal treatments, and sample collection has been previously reported by Abril-Parreño et al. [18].

Briefly, cervical mucus samples were collected from six ewe breeds with known differences in pregnancy rates following cervical AI using frozen–thawed semen. These were Suffolk (low fertility) and Belclare (medium fertility) in Ireland, Ile de France and Romanov (both with medium fertility) in France, and NWS and Fur (both with high fertility) in Norway. At the natural cycle, all ewes were checked twice daily for signs of estrus over a 6-day period using a teaser ram with an apron fitted (no semen/seminal plasma was allowed to be deposited into the vagina of the ewe). At the synchronized cycle, ewes were synchronized using intravaginal progestagen vaginal sponges (20-mg Flugestone Acetate; Chronogest vaginal sponges, Intervet, Boxmeer, The Netherlands), inserted on a random day of the cycle. After 14 days, the sponges were removed and ewes were treated with equine chorionic gonadotropin (400 IU; Intervet, Boxmeer, The Netherlands). We used this established protocol that works in >95% of ewes (during the breeding season) based on previous studies [19, 20]. Synchronized ewes were not heat checked as is the norm for most inseminated in fixed AI programmes, and cervical mucus was collected at a time (56 h) when ewes would normally be cervically artificially inseminated in time-fixed AI programmes using frozen–thawed semen. Cervical mucus was collected from each ewe at the follicular phase of both a synchronized (56-h post pessary removal) and a natural estrus cycle (12-h post detection of standing estrus), which was then replicated three times with the same ewes over a period of approximately 6 months (Figure 1). After each mucus collection, samples were transported to the laboratory (maximum time = 1 h) for assessment of cervical mucus properties (weight, viscosity, and color) following which the samples were stored at –20°C. Values of mucus weight, viscosity, and color as well as a more detailed description of the experimental model can be found at Abril-Parreño et al. [18]. Mucus samples were ranked according to viscosity at collection as assessed by the time in seconds for 4 µL of mucus to fill a Leja 20-µm deep chamber slide (IMV Technologies, L'Aigle, France). The more viscous mucus was, the longer it took to fill the chamber. A maximum of 420 s was allowed per sample for mucus to fill the chamber. Following thawing, samples were pooled according to viscosity post collection to ensure enough mucin for analysis. For the synchronized animals, each pool consisted of mucus from five animals (five ewes where their average viscosity was highest pooled together, then the next five and so on) of the same breed collected over three replicates ( Supplemental file 1 (l_abril-parreno_et_al_sialylated_cervical_mucins_sup_file_1_ioac077.xlsx)). Each pool was a total of 15 samples consisting of five ewes, each with one sample collected at each of three replicates/cycle. We then pooled mucus (1 pool = 15 samples) from the same five animals for the natural cycle using the same mucus viscosity ranking as the synchronized cycle. The three replicates were three separate cycles at both a natural and a synchronized cycle with one mucus collection at the follicular phase of each cycle. In all, the sample collections took ∼6 months to complete (3 synchronized cycles and 3 natural cycles = 6 cycles). Mucins were purified from cervical mucus samples using the described method in  Supplemental file 2 (l_abril-parreno_et_al_sialylated_cervical_mucins_sup_file2_ioac077.docx). Following slaughter to collect cervical tissue (experiment 3 and 4), the ovaries were assessed for the presence or absence of dominant follicles (without an active corpus luteum) and/or fresh ovulations as evident by a corpus hemorrhagicum. These structures were present in all the ewes of this study confirming they responded successfully to the sponge. For experiments 3 and 4, cervical tissue samples from two Irish ewe breeds (Suffolk and Beclare) and two Norwegian ewe breeds (NWS and Fur) at the follicular phase of both synchronized and natural estrus cycle were collected and later subjected to RNA-sequencing analysis. For this study, specific mucin and sialic acid related genes were interrogated from the data set generated in our RNA-sequencing analysis. To assess the percentage of the epithelium consisting of goblet cells we used cervical tissue sections from Suffolk, Belclare, Fur, and NWS at the follicular phase of both a synchronized and a natural estrus cycle.

Figure 1.

Experimental flow diagram of cervical tissue and mucus collection, sample preparation and analysis. NWS = Norwegian White Sheep. Exp. = experiment.

Experiment 1: Weak Anion Exchange Chromatography—Ultra-Performance Liquid Chromatography Analysis

The objective of this experiment was to profile the abundance of neutral and acidic O-glycans in one pooled sample for each breed and type of estrus cycle. One pooled sample for each of the six ewe breeds within each type of cycle (natural or synchronized) was used. Belclare breed at the synchronized cycle was not analyzed as there was insufficient amount of mucin remaining. O-glycans were released from purified mucins as described by Abril-Parreño et al. [21]. The purified mucin from cervical mucus was also used for the O-glycan analysis, which included ultra-performance liquid chromatography (UPLC), mass spectrometry, and exoglycosidases digestion panels [21]. 2AB labelled O-glycans were separated by AEC-UPLC using a Waters DEAE anion exchange, 75 × 7.5 mm i.d., 10-µm column on an Aquity H-Class HILIC-UPLC system (Waters Corporation, Milford, MA) coupled with a fluorescence detector (Waters Corporation, Milford, MA), which was set with excitation and emission wavelengths of 330 and 420 nm, respectively. Gradient separations were performed using a solvent A of 20% v/v acetonitrile (Sigma Aldrich, Ark-low, Co Wicklow, Ireland) and solvent B of 0.1M ammonium acetate buffer pH 7.0 in 20% v/v acetonitrile. Samples were resuspended in 50 µL of water and an injection volume of 20 µL was used in a flow rate of 750 µL per min over a 30 min run using the following gradient: 0–5 min—100% A, 5–20 min—100% → 0% A, 20–22.5 min—0% A, 22.5–23 min—0% → 100% A, 23–30 min—100% A. A fetuin O-glycan standard was used for calibration.

Experiment 2: sialic acid speciation analysis

The objective of this experiment was to assess the sialic acid species of cervical mucins from a total of six mucus pools for each ewe breed at both types of cycle, with a total of 72 samples (six mucus pools from the 6 ewe breeds at both a natural and synchronized estrus) in duplicate that generated data from 144 samples. Sialic acids were released from the purified cervical mucin samples (500 mg) using mild acid hydrolysis by incubation for 2 h at 80°C with 25 µL of 2M acetic acid. From each sample 5 µL were used for labelling of sialic acid using a LudgerTag DMB (1,2-diamino-4,5-methylenedioxybenzene) Sialic Acid Labelling kit (Ludger Limited, Culham Science Centre, Abingdon, UK). Samples were labelled with 20 µL of DMB reaction mixture, which were previously prepared using 0.7 mg of DMB and 0.4 mg sodium dithionite in mercaptoethanol (1.2M) for 3 h at 50°C. The labelling reactions were quenched by adding 475 µL of milliQ water to the samples, which were immediately frozen at –20°C. The sialic acid reference panel and the standards supplied with the Ludger Kit were also labelled with 20 µL of DMB reaction mixture.

Analysis was performed within 72 h after sample preparation to avoid DMB degradation (which occurs over time). The DMB labelled samples were separated by reverse phase (RP)UPLC analysis using a LudgerSep-uR2, 2.1 × 50 mm, 1.9-µm column on an Aquity H-Class HILIC-UPLC system (Waters Corporation, Milford, MA) coupled with a fluorescence detector (Waters Corporation, Milford, MA). Gradient separations were performed using a solvent A of 9:7:84 acetonitrile:methanol:Milli-Q water and solvent B of ACN. An injection volume of 5 µL was used in a flow rate of 250 µL/min over a 15 min run using the following gradient: 0–7 min—100% A, 7–7.5 min—100% → 10% A, 7.5–8 min → 10% A (flow rate 250 µL/min), 8–8.5 min—10% → 100% A (flow rate 250 µL/min), 8.5–15 min—100% A (flow rate 250 µL/min). The separation temperature was set at 30°C, whereas the sample temperature was 10°C. Excitation and emission wavelengths for fluorescence detection were λ= 373 nm and λ= 448 nm, respectively. Sialic acid reference panel provided by the Ludger kit was performed creating a chromatogram with seven peaks (peak 1 = 5-N-glycolyl (Neu5Gc); peak 2 = 5-N-acetyl (Neu5Ac); peak 3 = 5-N-acetyl-7-O-acetylneuraminic (Neu5,7Ac₂); peak 4 = 5-N-glycolyl-9-O-acetylneuraminic acid (Neu5Gc,9Ac); peak 5 = Neu5,8Ac₂ 5-N-acetyl-8-O-acetylneuraminic; peak 6 = 5-N-acetyl-9-O-acetylneuraminic (Neu5,9Ac₂);and peak 7 = Neu5,x,xAc₃), which were used to quantify the relative levels of the different species of sialic acid in each sample.

Experiment 3: gene expression analysis using RNA-sequencing

The objective of this experiment was to examine functional groups of genes related to mucin production and the expression of enzymes involved in sialic acid production and modification from an RNA-sequencing dataset describing the overall cervical gene expression analysis. Total RNA was extracted from frozen cervical biopsies (n = 38 at the natural cycle and 39 and the synchronized cycle) immersed in TRIzol reagent, which was homogenized using a homogenizer (Bio-gen Pro200 Homogenizer, Pro Scientific) in order to lyse the tissue. The RNA extraction was completed using the RNeasy Kit (Quiagen Ltd., Crawley, West Sussex, UK) according to the manufacturer's instructions. Total RNA concentration was quantified using the Nanodrop ND-1000 UV–Vis Spectophotometer (NanoDrop Technologies Inc., Wilmington, DE). Quality of RNA was ascertained with the use of 2100 Agilent Bioanalyzer (Agilent Technologies, Santa Clara, CA). RNA integrity number was >7 in all samples and RNA aliquots were frozen after extraction. RNA libraries were prepared for all cervical tissue samples (Illumina TruSeq Stranded mRNA Library preparation). All libraries were sequenced on an Illumina NovaSeq sequencer. Sequencing was performed for each sample at 2 × 150 bp paired end reads (50 M reads) as previously described [22].

Raw sequence data were assessed for quality using the software FastQC (v 0.11.8)  http://www.bioinformatics.babraham.ac.uk/projects/fastqc/). Data were quality and adapter trimmed using the BBDuk java package to trim Illumina adapter sequences and any low quality bases (Phred score < 20) from the 3′ end of sequence read pairs. Reads were aligned to the ovine genome Oar_v3.1 using the spliced transcripts alignment to a reference (STAR) aligner. A maximum of two mismatches with the reference genome were allowed and only uniquely mapped read pairs were retained for downstream analysis. Read counts overlapping all protein coding genes in the Oar_v3.1 Ensembl (v.95) annotations were estimated using featureCounts. To filter out lowly expressed genes, genes with less than one count per million in at least ten samples were discarded from the analysis. Remaining gene counts were normalized uses the median of ratios method as implemented in DeSeq2 (version 1.130.0) [23] to account for varying sequencing depth between samples.

Experiment 4: histological analysis of cervical goblet cells

The objective of this experiment was to assess the percentage of cervical goblet epithelial cells in the cervical tissue of four breeds with known differences in pregnancy rates following cervical AI with frozen–thawed semen. Additional formalin fixed cervical biopsies (randomly chosen) were paraffin-embedded, sectioned at 5-µm thickness, mounted on glass slides and stained with periodic acid Schiff (PAS) and Alcian blue (AB, pH 2.5) to assess the presence of goblet cells in the cervical epithelium by an experienced histology expert according to the method used by Pluta et al. [24]. Previous stain with PAS, the sections were deparaffinised and oxidized in 1% periodic acid for 10 min, followed by several rinses in distilled water. Staining was carried out in Schiff reagent at 4°C for 15 min followed by rinsing in distilled water. Sections were then counter stained with hematoxylin for 1 min, washed, dehydrated, and mounted. Sections stained with AB pH 2.5 were previously deparaffinised and stained for 5 min with 1% AB in 3% acetic acid pH 2.5, followed by rinsing several times in distilled water. After counterstaining with 0.5% aqueous neutral red for 1 min, sections were washed, dehydrated and then mounted. We used 3–5 animals per breed. The percentage of goblet cells (cells stained in blue) was determined by counting the number of these cells in a delimited area (10 replicates per slide). Slides from both stains were analyzed using Image-Pro Premium 9.2 by Media Cybernetics (Marlow, Buckinghamshire, UK).

Experiment 1: WAX analysis; high fertility ewe breeds have higher concentration of nonsialylated glycans in cervical mucins

The majority (75%) of the structures was in the neutral fraction (S0 fraction), containing nonsialylated glycans across the six ewe breeds at both the natural and synchronized cycle. In our previous study published [25], the overall O-glycan analysis demonstrated that ∼60% of the total glycans were neutral structures, which supports the overall trends of the present experiment. At the synchronized cycle, NWS (high fertility) had the highest percentage of nonsialylated glycans, whereas at the natural estrus cycle Fur (high fertility) had the highest. However, these were followed by the low fertility, Suffolk, which also had a high percentage of nonsialylated structures at the synchronized cycle. Levels of charged fractions, containing mono-, di-, and tri-sialylated O-glycans are also shown in Table 1.

Experiment 2: sialic acid speciation analysis identified the highest levels of Neu5,9Ac₂ in the low fertility Suffolk breed

Relative quantification of the detected sialic acids demonstrated that there were two major peaks corresponding to 5-N-glycolyl- (Neu5Gc) and 5-N-acetyl- (Neu5Ac); which were glycolylated and acetylated, respectively. These two major peaks represented 90–94% of the total sialic acid content of each sample. Minor peaks corresponding to 5-N-acetyl-7-O-acetylneuraminic (Neu5,7Ac₂); 5-N-glycolyl-9-O-acetylneuraminic acid (Neu5Gc,9Ac); 5-N-acetyl-8-O-acetylneuraminic Neu5,8Ac₂; 5-N-acetyl-9-O-acetylneuraminic (Neu5,9Ac₂); and Neu5,x,xAc₃ were also detected ( Supplemental Figure S1 (l_abril-parreno_et_al_sialylated_cervical_mucins_sup_fig_ioac077.docx)).

There was no interaction between ewe breed and type of cycle (P > 0.05) for any of the detected sialic acids. Despite Neu5x,xAc₃ being the least prevalent sialic acid detected there was a higher content at the natural cycle compared with the synchronized cycle (2.84 ± 0.49 and 1.56 ± 1.07, respectively; P < 0.05). There was an effect of ewe breed on Neu5Gc, Neu5Ac, Neu5,7Ac₂, Neu5Gc,9Ac_, Neu5,8Ac₂, and Neu5,9Ac₂ (P < 0.05, Figure 2). At a natural estrus, Suffolk had a lower concentration of Neu5Gc compared with Romanov (P < 0.05). Regarding the acetylated species, Suffolk and Ile de France had higher abundance of Neu5Ac compared with Romanov (P < 0.001). Belclare had lower concentration of Neu5,7Ac₂ compared with Fur ewes (P < 0.05). Ile de France had lower abundance of Neu5Gc,9Ac than Fur and NWS (P < 0.05). However, Ile de France had higher proportion of Neu5,8Ac₂ compared with Belclare (P < 0.05). In addition, Romanov had the lowest concentration of Neu5,9Ac₂, showing significant differences with Suffolk, Belclare, Ile de France, and Fur. The low fertility Suffolk breed had the highest concentration of Neu5,9Ac₂, and was higher than both Ile de France (medium fertility) and NWS (high fertility; P < 0.05) at both types of cycle.

Experiment 3: the cervical expression of mucin and sialic acid related genes is affected by ewe breed and type of estrus cycle

Differential gene expression analysis indicated that ewe breed, type of the cycle and their interaction was associated with extensive alterations in cervical gene expression at the follicular phase of the estrus cycle.

Sialyltransferases

The sialyltransferases are a representative group that catalyze the transfer of sialic acids to the glycan structure. There were 14 sialyltransferases expressed in sheep cervical tissue at the follicular phase of both types of cycle (natural and synchronized), these were ST3GAL1, ST3GAL2, ST3GAL3, ST3GAL4, ST3GAL5, ST3GAL6, ST6GAL1, ST6GAL2, ST6GALNAC1, ST6GALNAC2, ST6GALNAC3, ST6GALNAC4, ST8SIA2, and ST8SIA4.

Table 1.

Relative percentage area (%) derived from the UPLC total profile of nonsialylated (Fraction S0), mono-sialylated (Fraction S1), di-sialylated (Fraction S2), and tri-sialylated (Fraction S3) O-glycans in cervical mucin from six ewe breeds (Suffolk, Belclare, Ile de France, Romanov, Fur, and Norwegian White Sheep (NWS)) at the follicular phase of both a natural and a synchronized estrus cycle. One pooled samples per breed and type of cycle was analyzed by weak Anion exchange chromatography (WAX)—ultra-performance liquid chromatography (UPLC) analysis

Figure 2.

Relative percentage area derived from the UPLC total profile of seven sialic acid species (Neu5Gc, Neu5Ac, Neu5,7Ac₂, Neu5Gc,9Ac, Neu5,8Ac₂, Neu5,9Ac₂, and Neu5,x,xAc3) in cervical mucins at the follicular phase of a synchronized (A) and a natural estrus cycle (B) from Suffolk (low fertility) Belclare, Ile de France, Romanov (all medium fertility), Fur and Norwegian White Sheep (NWS; both high fertility) ewes as assessed using RP–ultra-performance liquid chromatography (UPLC). Peak data were analyzed using a multivariate analysis of variance (MANOVA) with post-hoc analysis using Tukey's Honest Significant difference test. Values are mean ± SEM. ^abc Different superscripts differ significantly within sialic acid species (P < 0.05).

The ST3 β-Galactoside α-2,3-Sialyltransferase 3 (ST3GAL3) that catalyzes the formation of the Neu5Ac-α-2,3-Gal-β-1,3-GlcNAc, had lower expression in Suffolk compared with NWS (highest fertility) at the synchronized cycle (P < 0.05; Figure 5). ST3GAL4, which catalyzes the formation of the Neu5Ac-α-2,3-Gal-β-1,4-GlcNAc and Neu5Ac-α-2,3-Gal-β-1,3-GlcNAc, had lower expression in the low fertility Suffolk compared with the high fertility Fur and NWS at the synchronized cycle (P < 0.05). ST6 β-Galactoside α-2,6-Sialyltransferase 1 (ST6GAL1) transfers sialic acid from the donor of substrate CMP-sialic acid to galactose containing acceptor substrates. There was higher expression in Suffolk compared with Belclare and Fur at the synchronized cycle (P < 0.05). In addition, ST6GAL2 presented higher expression in Suffolk compared with the other three breeds (Belclare, Fur, and NWS) at a synchronized cycle (P < 0.05). ST8SIA2 is involved in polysialic acid synthesis by adding α-2,8-linkages to the α-2,3-linked and α-2,6-linked sialic acid of glycans. There was higher expression of ST8SIA2 in the low fertility Suffolk breed compared with Fur ewes at both a natural and a synchronized cycle (P<0.05).

Sialic acid-specific O-acetylesterases

Sialic acid-specific O-acetylesterases, including the SIAE gene, remove 9-O-acetylation modifications from sialic acids and thus permits α-2,6 linked sialic acid on N-glycans on B cell glycoproteins to interact with CD22/SIGLEC2, a sialic acid-binding lectin that can inhibit B cell antigen receptor signaling. In our study, there were no differences in the expression of SIAE between ewe breeds at either a natural or synchronized cycle (P > 0.05). However, CD22 had over twofold increased expression (FC = 2.71) in Suffolk compared with NWS at the synchronized cycle (P < 0.05).

Figure 3.

Expression of genes (read counts) at the follicular phase of a synchronized estrus cycle in Suffolk, Belclare, Fur, and Norwegian White Sheep (NWS). Transcript counts were modelled by fitting the data to a negative binomial distribution using genewise dispersion estimates and differentially expressed genes were identified with a generalized linear model likelihood ratio test. Statistical tests were corrected for multiple testing using the Benjamini–Hochberg method. Significant differences (P < 0.05) between the reference level (Suffolk) and the other ewe breeds are denoted with a * symbol.

Figure 4.

Expression of genes (read counts) at the follicular phase of a natural estrus cycle in Suffolk, Belclare, Fur, and Norwegian White Sheep (NWS). Transcript counts were modelled by fitting the data to a negative binomial distribution using genewise dispersion estimates and differentially expressed genes were identified with a generalized linear model likelihood ratio test. Statistical tests were corrected for multiple testing using the Benjamini–Hochberg method. Significant differences (P < 0.05) between the reference level (Suffolk) and the other ewe breeds are denoted with a * symbol.

Experiment 4: the percentage of goblet cells differs between high and low fertility ewe breeds under the effect of estrus synchronization

There was a type of the cycle (natural versus synchronized) by ewe breed interaction on the percentage of goblet cells (P < 0.05; Figure 7). During the natural cycle, Belclare ewes had the lowest percentage of goblet cells and it was lower than in Suffolk, Fur, and NWS (P < 0.05). However, in the synchronized cycle, Suffolk ewes presented the lowest percentage of goblet cells, which was lower compared with Belclare, Fur, and NWS ewes (P < 0.05). There were no differences between both Norwegian ewe breeds (Fur and NWS) with the natural cycle whereas, during the synchronized cycle Fur ewes had a higher percentage of goblet cells in the cervical epithelium than NWS (P < 0.05). The effect of estrus synchronization was also evident as Suffolk had a lower percentage of goblet cells than Fur and NWS at the synchronized cycle (P < 0.05) although there were no differences between them at the natural cycle (P > 0.05).