Genotyping of rams based on melatonin receptor 1A gene polymorphisms: a tool in sire selection?

Animals

Eighteen Rasa Aragonesa rams of proven fertility were used in this study. The rams belonged to the Asociación Nacional de Criadores de Ganado Ovino Selecto de Raza Rasa Aragonesa (ANGRA), were housed in the facilities of the Centro de Selección y Reproducción Animal (CENSYRA, Centro de Transferencia Agroalimentaria, Movera, Zaragoza, Spain) and were used routinely for field AI in commercial farms.

All animal procedures were performed in accordance with the Spanish Animal Protection Regulation 348/2000 which conforms to European Union Regulation 98/58/CE. Approval from the Ethics Committee of the University of Zaragoza was not a prerequisite for this study since we worked with semen or blood samples.

Genotyping

Blood samples were collected from each ram from the jugular vein using sterile vacuum tubes (BD Vacutainer Systems, Belliver Industrial Estate, Plymouth, UK) with ethylenediamine tetraacetic acid (EDTA) as an anticoagulant. The blood samples were aliquoted in aliquots of 200 μL and stored at −20°C until analysis. DNA was extracted from an aliquot of whole blood using a commercial DNA extraction kit (NucleoSpin Blood Mini Kit, Macherey–Nagel, Dueren, Germany). After extraction, both DNA quantity and purity were assessed using a Nanodrop1000 Spectrophotometer (Thermo Scientific, Waltham, MA, USA). The amount of DNA obtained was quantified by measuring the absorbance at 260 nm, and purity was determined by evaluating the A₂₆₀/A₂₈₀ and A₂₆₀/A₂₃₀ ratios.

To amplify the region of the Exon II where the RsaI and MnlI polymorphisms are located, we used the set of primers (forward: TCCCTCTGCTACGTGTTCCT; reverse: GTTTGTTGTCCGGTTTCACC) following Calvo et al. (2018). The fragments were amplified by PCR in a final volume of 50 μL of a reaction mix that contained 5.0 μL of 10 × Reaction Buffer MgCl₂ FREE (Biotools, B&M Labs, Madrid, Spain), 1.0 μL of 10 pM of each primer, 1.0 μL of 200 nM dNTPs, 2.0 μL of 50 mM MgCl₂ solution (Biotools, B&M Labs, Madrid, Spain) and 1 U of Pfu DNA polymerase (Biotools, B&M Labs, Madrid, Spain). When the DNA concentration obtained was lower than 20 ng/μL, an EmeraldAmp® GT PCR Master Mix (Takara Bio, Kusatsu, Japan) was used, following the manufacturer’s indications. The PCR conditions were the following: initial denaturation step at 94°C for 3 min; 35 cycles of 94°C for 1 min, the annealing temperature (58°C for the pair of primers above) for 1 min, and 72°C for 1 min, with a final extension step at 72°C for 10 min. The PCR products were confirmed by electrophoresis in 1 × TBE buffer on a 1.7% (w/v) agarose gel containing 5 μL of SYBR™ Safe DNA Gel Stain (Invitrogen, Waltham, MA, USA) parallel with a 100 bp marker (GeneRuler 100 bp DNA Ladder, Thermo Scientific, Waltham, MA, USA) at a constant voltage of 110 V for 40 min. The bands obtained were then displayed using an ultraviolet light trans-illuminator (BioRad Gel Doc XR Imaging System, Hercules, CA, USA).

All PCR products were purified and sequenced in both directions by a commercial sequencing service (STAB VIDA, Lda., Caparica, Portugal). The Blast algorithm (www.ncbi.nlm.nih.gov/blast/) was used to compare the sequences obtained with the genome version Oar_rambouillet_v1.0 (GenBank assembly accession number: GCF_002742125.1). Nucleotide sequence alignments were carried out using the BioEdit Sequence Alignment Editor software (www.mbio.ncsu.edu/BioEdit/BioEdit). Finally, the sequences were analysed with FinchTV software ver. 1.4. (finchtv.software.informer.com/1.4/).

Semen collection and transport

The rams were in a regular semen collection regime, of at least one weekly collections since they are the sires used to carry out inseminations on the farms of the association’s members. Ram ejaculates were collected individually using an artificial vagina by the staff of the center where the animals were housed. After collection, a routine semen assessment was performed in the semen collection facilities, which included the volume of the ejaculate (measured in the graduated collection tube); concentration measured with a spectrophotometer (AccuRead, IMV Technologies, L’Aigle, France); mass motility scored from 0 to 5 and assessed by optical microscopy at 100× magnification; and the proportion of motile spermatozoa (evaluated with a CASA system, AI Station, Sperm Analysis Technologies S.L, Buñol, Valencia, Spain). Thereafter, semen was diluted to 1.6 × 10⁹ spermatozoa/mL with INRA 96 (Imv Technologies, L’Aigle, France), put into 0.5-mL straws and refrigerated at 15°C for transport. Once a month throughout a whole year (from September to August), refrigerated semen samples from the 18 rams were sent to the facilities of the University of Zaragoza. Once the samples arrived at the laboratory, an extensive semen quality analysis was performed, which included sperm motility, morphology, membrane integrity, intracellular levels of reactive oxygen species (ROS), phosphatidylserine (PS) inversion, DNA fragmentation and capacitation status.

Sperm motility analysis

Motility parameters (percentages of motile (TM) and progressive motile (PM) spermatozoa) were measured using a computer-assisted CASA system (ISAS 1.0.4; Proiser SL, Valencia, Spain) as described previously (Gimeno-Martos et al. 2019). Sperm motility was recorded with a video camera (Basler A312f, Basler AG, Ahrensburg, Germany) mounted on a microscope (Nikon Eclipse 50i, Nikon Instruments Inc., Tokyo, Japan) equipped with a 10× negative-phase contrast lens. Samples were diluted 1:15 in a medium with the following composition: 0.25 M sucrose, 100 mM EGTA, 0.5 mM sodium phosphate, 50 mM glucose, 100 mM HEPES and 20 mM KOH. A drop of 8 μL of each diluted sample was placed between a pre-warmed slide and coverslip and kept at 37°C in a heated slide holder during analysis. Five videos at 25 frames/s for 1 s were recorded for each sample. The CASA system settings for the analysis were the following:

Particle area (μm²): 3 (min)−70 (max); VCL (μm/s): 10 > slow > 45 > medium > 75 > rapid; Progressive (% STR): 80; Connectivity: 12.

Sperm morphology evaluation

Semen samples were diluted 1:6 in the aforementioned medium before being mixed (10 μL) with 5 μL eosin and 5 μL nigrosine (Ax et al. 2000). After mixing, 20 μL of the stained sample were placed on a slide and spread with the help of another one. Smears were air-dried and then observed by bright-field microscopy using a Nikon Eclipse E-400 microscope (Kanagawa, Japan). At least 200 spermatozoa were analysed for each sample at 1000× magnification to determine the percentage of normal morphology cells. Sperm cells that showed a detached head, bent tail, coiled tail or proximal or distal droplet were considered abnormal (Ax et al. 2000).

Flow cytometry analyses

Flow cytometry measurements were performed using a Beckman Coulter FC 500 flow cytometer (Beckman Coulter Inc., Fullerton, CA, USA) equipped with two lasers of excitation (argon-ion laser, 488 nm; and solid-state laser, 633 nm), five filters of absorbance (FL1-525, FL2-575, FL3-610, FL4-675 and FL5-755; ±5 nm each bandpass filter) and the CXP software. A flow rate stabilised at 200–300 cells/s was used, and a minimum of 20,000 events were recorded in all experiments. The sperm population was gated for further analysis based on its specific forward (FS) and side scatter (SS) properties to exclude other non-sperm events.

Capacitation status

The capacitation status was determined using chlortetracycline (CTC) staining (Ward and Storey 1984). A CTC solution (750 μM) was prepared on the day of each experiment in a buffer containing 20 mM Tris, 130 mM NaCl and 5 μM cysteine (pH 7.8), and then passed through a 0.22-μm filter. For the analysis, 20 μL of each diluted sample (dilution 1:6) was mixed with 20 μL of CTC solution and fixed with 5 μL of 1.25% (w/v) paraformaldehyde in 0.5 M Tris–HCl (pH 7.8). Samples were incubated at 4°C in the dark for at least 30 min. After incubation, a 4-μL aliquot of the stained sample was placed on a glass slide and mixed with 2 μL of 0.22 M triethylenediamine (DABCO) in glycerol : PBS (9:1, v/v) at RT and semi-darkness. Samples were then covered with 24 × 48-mm coverslips, sealed with nail polish, and stored in the dark at −20°C. Samples were examined using a Nikon Eclipse E-400 microscope (Kanagawa, Japan) under epifluorescence illumination using a V-2A filter to evaluate CTC patterns, and 200 spermatozoa were scored per slide. Sperm classification followed Gillan et al. (1997) as follows: non-capacitated spermatozoa (NC, with even yellow fluorescence over the head, with or without a bright equatorial band); capacitated cells (C, with fluorescence on the acrosome) and acrosome-reacted cells (R, without fluorescence on the head and with or without a bright equatorial band).

Statistical analysis

Data are shown as mean ± s.e.m. The effect of the season (reproductive season: from September to February; non-reproductive season: from March to August) and RsaI and MnlI polymorphism on seminal quality was evaluated by mixed ANOVA. First, possible outliers were identified by the ROUT method (Motulsky and Brown 2006). The normality of the data was assessed by the Kolmogorov–Smirnov test, and then values were normalised by arcsine transformation. The homogeneity of variances was assessed by Levene’s test. For the mixed ANOVA, the season was considered the ‘within-subjects’ factor, whereas the RsaI and MnlI genotypes were the ‘between-subjects’ factors. For post hoc analyses, Tukey’s multiple comparisons test or Dunn’s method was used when homoscedasticity and heteroscedasticity were detected, respectively. Statistical analyses were performed with SPSS Statistics ver. 26 (IBM Analytic, Armonk, NY, USA) and GraphPad Prism ver. 8 (La Jolla, CA, USA).

Genotypes of the rams used in the study

The result of ram genotyping is shown in Table 1. For the RsaI polymorphism, nine rams were C/C, five rams were C/T and four were T/T. For the MnlI polymorphism, seven of them were G/G, 7 G/A and 4 A/A. Three genotypes (T/T*G/A, C/T*A/A and T/T*A/A) were not present.

Interaction between RsaI, MnlI and season

A summary of the results of mixed ANOVA is shown in Table 2. No statistically significant three-way interaction between RsaI, MnlI and season, or two-way interaction between season and RsaI or MnlI, was found in any seminal quality parameters analysed. Nevertheless, we found a significant two-way interaction between RsaI and MnlI for total motility, cell membrane integrity (viability) and viable spermatozoa with low ROS. There was also a main effect of the RsaI genotype for total motility, viability, viable spermatozoa with low ROS, viable spermatozoa without PS translocation and DNA intact spermatozoa, and the MnlI genotype for viability, viable spermatozoa with low ROS and viable spermatozoa without PS translocation.

We likewise detected a seasonal effect on total and progressive motility, viability, viable spermatozoa with low ROS, capacitation status and DNA fragmentation. Due to this seasonal effect on most of the studied parameters, further results were separated between reproductive and non-reproductive seasons. Only significant results (i.e. total motility, viability, viable spermatozoa with low ROS, viable spermatozoa without PS translocation and DNA fragmentation) are described below, and non-significant values (progressive motility, capacitation status and morphology) are shown in the supplementary material (Tables S1, S2 and S3).

Effect of RsaI polymorphism on sperm quality

The seminal quality of T/T rams was lower than the other genotypes. Thus, these males presented a lower percentage of motile, membrane intact, viable with low ROS or without PS translocation and DNA intact spermatozoa than C/C or C/T rams. However, these differences were higher in reproductive than in the non-reproductive season and were not detected for total motility or the percentage of spermatozoa without PS translocation during the non-reproductive season (Fig. 1). The other two genotypes, C/C and C/T, did not show any statistical differences between them.

Fig. 1.

Percentage of total motile (a), viable (b), viable with low ROS levels (c), viable without PS translocation (d) and DNA intact (e) spermatozoa in semen samples from animals carrying different RsaI genotypes (C/C = nine rams; C/T = five rams; and T/T = four rams) during the reproductive season (RS) and the non-reproductive season (NRS). Data are shown as mean ± s.e.m. (n = number of rams of each genotype × 6 semen samples per season). *P < 0.05; **P < 0.01 and ***P < 0.001.

Effect of MnlI polymorphism on sperm quality

When the effect of the MnlI polymorphism was evaluated, we found a higher percentage of viable spermatozoa, viable sperm with low ROS and viable cells without PS translocation in samples from G/A rams (Fig. 2). These differences were also higher in the reproductive season but for viable spermatozoa with low ROS. No differences were found for total motility and DNA integrity in any season.

Fig. 2.

Percentage of total motile (a), viable (b), viable with low ROS levels (c), viable without PS translocation (d) and DNA intact (e) spermatozoa in semen samples from animals carrying different MnlI genotypes (G/G = seven rams; G/A = seven rams; and A/A = four rams) during the reproductive season (RS) and the non-reproductive season (NRS). Data are shown as mean ± s.e.m. (n = number of rams of each genotype × 6 semen samples per season). *P < 0.05; **P < 0.01 and ***P < 0.001.

Effect of the combination of RsaI and MnlI polymorphisms on sperm quality

Since mixed ANOVA analysis had detected a significant interaction between RsaI and MnlI polymorphisms in total motility, viability and viable spermatozoa with low ROS (Table 2) and a significance of P = 0.062 in viable sperm without PS translocation, it was essential to study the effect of the combination of both polymorphisms on seminal quality.

The results showed that, within the G/G males, those that also carried the T/T genotype for RsaI had worse semen quality than the G/G*C/C and the G/G*C/T (Fig. 3). The same was observed, albeit to a lesser extent, in males that carried the A/A genotype for MnlI within the C/C males for RsaI.

Fig. 3.

Percentage of total motile (a), viable (b), viable with low ROS levels (c), viable without PS translocation (d) and DNA intact (e) spermatozoa in semen samples from animals carrying different combinations of RsaI and MnlI polimorphysms (C/C*G/G = one ram; C/T*G/G = two rams; T/T*G/G = four rams; C/C*G/A = four rams; C/T*G/A = three rams; and C/C*A/A = four rams) during the reproductive season (RS) and the non-reproductive season (NRS). Data are shown as mean ± s.e.m. (n = number of rams of each genotype × 6 semen samples per season). *P < 0.05; **P < 0.01 and ***P < 0.001.

Given that no differences in seminal quality had been observed between males that were not T/T or A/A, in order to avoid the problem of the small number of animals with some combinations of alleles, data were grouped to compare the effect on seminal quality of carrying the lowest frequency alleles in homozygosity (T/T or A/A).

The results revealed that rams carrying the T/T or A/A genotype, regardless of their genotype for the other polymorphism, presented lower seminal quality, especially for viability, viable sperm with low ROS and viable cells without PS translocation (Fig. 4). Moreover, differences were more significant for T/T rams than A/A rams and during the reproductive season. T/T rams also showed differences in motility. No differences were found for DNA-intact spermatozoa.

Fig. 4.

Percentage of total motile (a), viable (b), viable with low ROS levels (c), viable without PS translocation (d) and DNA intact (e) spermatozoa in semen samples from animals carrying the C/C*A/A genotype (n = four rams); the T/T*G/G genotype (n = four rams) and the other possibilities of genotypes (C/•*G/•, n = 10 rams) during the reproductive season (RS) and the non-reproductive season (NRS). Data are shown as mean ± s.e.m. (n = number of rams × 6 semen samples per season). *P < 0.05; **P < 0.01 and ***P < 0.001.