ABSTRACT
Artificial insemination success in swine is mainly associated with semen dose quality. Thus, this study compared quality control parameters in 11 Brazilian boar studs after applying audit services for 24 months (1,650 boars). An extensive checklist was applied in each audit, registering ‘compliance’ or ‘noncompliance’ for 75 items. Semen doses produced were analyzed as regards volume and sperm concentration, and microbiological analyses were conducted for semen and water samples collected at distinct production stages. On average, boar studs produced 112.9 semen doses per boar per month, and the odds of raw semen contamination increased when boars were inadequately housed and doses were collected under increased temperatures, with no anti-slip rubber mat or after a poor prepuce cleaning (p < 0.05). Collection from boars with locomotor problems and no regular change of reverse osmosis filters increased the contamination odds in semen doses produced and stored at the stud (p < 0.05). As regards the water submitted to the osmosis reverse process, contamination odds increased as a result of deficient cleaning and disinfection of the purification equipment (p < 0.05). Risk factors for reduced sperm motility (< 70 %) were: no anti-slip rubber mat for semen collection, no cleaning program for automatic feeding system (drops) and bins, and inadequate intervals between semen collections (≤ 2 days or > 7 days; p < 0.05). Two boar studs had the best results for compliance with the checklist items. Constant monitoring, appropriate hygiene of facilities and equipment, and periodical staff training are highlighted as non-negotiable points for boar semen dose quality.
bacterial contamination; benchmarking; boar semen; semen doses; sperm quality
Introduction
Artificial insemination (AI) in swine offers several advantages, such as genetic gains, sanitary security, reduced breeding costs, better use of facilities, etc. (Bortolozzo et al., 2005Bortolozzo FP, Wentz I, Dallanora D. 2005. Present situation of artificial insemination in swine. Acta Scientiae Veterinariae 33: 17-32 (in Portuguese, with abstract in English). https://doi.org/10.22456/1679-9216.14429
https://doi.org/10.22456/1679-9216.14429...
). Nowadays more than 90 % of females worldwide are mated through AI, presenting satisfactory reproductive performance (Waberski et al., 2019Waberski D, Riesenbeck A, Schulze M, Weitze KF, Johnson L. 2019. Application of preserved boar semen for artificial insemination: Past, present and future challenges. Theriogenology 137: 2-7. https://doi.org/10.1016/j.theriogenology.2019.05.030
https://doi.org/10.1016/j.theriogenology...
). Most AI procedures in swine are performed with cooled semen stored at 15-18 °C for 3-7 days (Waberski et al., 2019Waberski D, Riesenbeck A, Schulze M, Weitze KF, Johnson L. 2019. Application of preserved boar semen for artificial insemination: Past, present and future challenges. Theriogenology 137: 2-7. https://doi.org/10.1016/j.theriogenology.2019.05.030
https://doi.org/10.1016/j.theriogenology...
; Mellagi et al., 2023Mellagi APG, Will KJ, Quirino M, Bustamante-Filho IC, Ulguim RR, Bortolozzo FP. 2023. Update on artificial insemination: semen, techniques, and sow fertility. Molecular Reproduction and Development 90: 601-611. https://doi.org/10.1002/mrd.23643
https://doi.org/10.1002/mrd.23643...
), and the AI success has been associated mainly with boar semen dose quality (Bortolozzo et al., 2015 Bortolozzo FP , Menegat MB , Mellagi APG , Bernardi ML , Wentz I . 2015. New artificial insemination technologies for swine. Reproduction in Domestic Animals 50: 80-84. https://doi.org/10.1111/rda.12544
https://doi.org/10.1111/rda.12544...
; Knox, 2016Knox RV, 2016. Artificial insemination in pigs today. Theriogenology 85: 83-93. https://doi.org/10.1016/j.theriogenology.2015.07.009
https://doi.org/10.1016/j.theriogenology...
).
Boar semen processing spans several steps; therefore, the quality produced can be associated with many factors (Rodriguez et al., 2017 Rodriguez AL , Van Soom A , Arsenakis I , Maes D . 2017. Boar management and semen handling factors affect the quality of boar extended semen. Porcine Health and Management 3: 15. https://doi.org/10.1186/s40813-017-0062-5
https://doi.org/10.1186/s40813-017-0062-...
), such as bacterial contamination (Wolff et al., 1993Wolff H, Panhans A, Stolz W, Meurer M. 1993. Adherence of Escherichia coli to sperm: a mannose mediated phenomenon leading to agglutination of sperm and E. coli. Fertility and Sterility 60: 154-158. https://doi.org/10.1016/S0015-0282 (16)56054-3
https://doi.org/10.1016/S0015-0282 (16)5...
; Prieto-Martínez et al., 2014Prieto-Martínez N, Bussalleu E, Garcia-Bonavila E, Bonet S, Yeste M. 2014. Effects of Enterobacter cloacae on boar sperm quality during liquid storage at 17 °C. Animal Reproduction Science 148: 72-82. https://doi.org/10.1016/j.anireprosci.2014.05.008
https://doi.org/10.1016/j.anireprosci.20...
; Nitsche-Melkus et al., 2020Nitsche-Melkus E, Bortfeldt R, Jung M, Schulze M. 2020. Impact of hygiene on bacterial contamination in extended boar semen: an eight-year retrospective study of 28 European Al centers. Theriogenology 146: 133-139. https://doi.org/10.1016/j.theriogenology.2019.11.031
https://doi.org/10.1016/j.theriogenology...
) and the temperature control over the semen processing, transport and storage of semen doses (Schulze et al., 2013Schulze M, Henning H, Rüdiger K, Wallner U, Waberski D. 2013. Temperature management during semen processing: Impact on boar sperm quality under laboratory and field conditions. Theriogenology 80: 990-998. http://dx.doi.org/10.1016/j.theriogenology.2013.07.026
http://dx.doi.org/10.1016/j.theriogenolo...
). Because of these variables, boar studs require systematic quality control of semen processing, identifying and controlling the risk factors for decreased semen quality, which can be obtained through the implementation of Hazard Analysis and Critical Control Points (HACCP) systems, as prescribed for bull studs in Brazil (Goularte et al., 2015Goularte KL, Madeira EM, Ferreira CER, Duval EH, Vieira AD, Mondadori RG, et al. 2015. Hazard analysis and critical control points system for a bull semen production centre. Reproduction in Domestic Animals 50: 972-979. https://doi.org/10.1111/rda.12617
https://doi.org/10.1111/rda.12617...
). It is noteworthy that quality control programs also promote the proper characterization of studs (Knox et al., 2008Knox RV, Levis D, Safranski T, Singleton W. 2008. An update on North American boar stud practices. Theriogenology 70: 1202-1208. https://doi.org/10.1016/j.theriogenology.2008.06.036
https://doi.org/10.1016/j.theriogenology...
; Bennemann et al., 2020Bennemann PE, Bragança JFM, Walter MP, Bottan J, Machado SA. 2020. Characterization of boar studs in Brazil. Ciência Rural 50: e20190998. https://doi.org/10.1590/0103-8478cr20190998
https://doi.org/10.1590/0103-8478cr20190...
), as well as the setting of benchmarks, which are critical points for further improving the quality of boar semen doses.
The implementation of an HACCP system for boar studs has already been reported (Riesenbeck et al., 2015 Riesenbeck A , Schulze M , Rüdiger K , Henning H , Waberski D . 2015. Quality control of boar sperm processing: implications from European AI centres and two spermatology reference laboratories. Reproduction in Domestic Animals 50: 1 - 4 . https://doi.org/10.1111/rda.12573
https://doi.org/10.1111/rda.12573...
; Schulze et al., 2015Schulze M, Ammon C, Rüdiger K, Jung M, Grobbel M. 2015. Analysis of hygienic critical control points in boar semen production. Theriogenology 83: 430-437. https://doi.org/10.1016/j.theriogenology.2014.10.004
https://doi.org/10.1016/j.theriogenology...
), and to date, 40 European boar studs have been submitted to a solid science-based quality control program (Schulze et al., 2022 Schulze M , Jung M , Hensel B . 2022. Science-based quality control in boar semen production. Molecular Reproduction and Development 90: 612-620. https://doi.org/10.1002/mrd.23566
https://doi.org/10.1002/mrd.23566...
). In Brazil, 42 boar studs are currently subject to the guidelines required by official agencies (MAPA, 2020), producing more than 9.5 million semen doses per year that results in an annual production of 4.9 million ton of pork (Bennemann et al., 2018Bennemann PE, Machado SA, Girardini LK, Sonálio K, Tonin AA. 2018. Bacterial contaminants and antimicrobial susceptibility profile of boar semen in southern Brazil studs. Revista MVZ Córdoba 23: 6637-6648. https://doi.org/10.21897/rmvz.1338
https://doi.org/10.21897/rmvz.1338...
; ABPA, 2023). Nevertheless, standardized quality control programs still have to be applied to Brazilian boar studs. Additionally, the little available information regarding Brazilian boar studs focuses mainly on the facilities and workflow process (Bennemann et al., 2020Bennemann PE, Bragança JFM, Walter MP, Bottan J, Machado SA. 2020. Characterization of boar studs in Brazil. Ciência Rural 50: e20190998. https://doi.org/10.1590/0103-8478cr20190998
https://doi.org/10.1590/0103-8478cr20190...
).
The data above reinforce that there is still room for characterizing Brazilian boar studs and identifying, monitoring, and controlling the critical issues of quality control programs. Therefore, this study aimed to implement a quality control system to evaluate routine practices in Brazilian boar studs, assessing critical points for semen dose quality and comparing the studs according to their compliance level.
Materials and Methods
Audits in boar studs
This study included data from 11 boar studs from five Brazilian states located in the mid-western and southern regions (Mato Grosso, Mato Grosso do Sul, Paraná, Santa Catarina, and Rio Grande do Sul), comprising records from 1,650 boars. The studs were periodically visited through the same systems of veterinary services for 24 months, totalizing 96 audits (53 audits in the autumn and winter, and 43 audits in the spring and summer). During each audit, a checklist containing 75 items was applied. The items were grouped into eight categories: boar housing; boar health; semen collection; laboratory structure; semen processing; semen quality; water quality; and cleaning and disinfection (Table 1), and were classified as compliant or noncompliant. The studs’ general characteristics are summarized in Table 2.
Semen collection and processing
In all studs, boar semen was collected via a semi-automatic collection system (Magapor). After collection, ejaculate was processed and semen doses were produced with a long-term extender (Vitasem®, Magapor). They were stored in the boar stud and then transported to the destination farm at 16-18 °C. For each ejaculate collected, boar identification, date of collection, raw semen volume, number of semen doses produced, and type of semen dose (either for cervical AI, CAI; or post-cervical AI, PCAI) were recorded. The target volume for CAI and PCAI semen doses was 80 mL and 45 mL, respectively. Sperm motility, concentration, and morphological abnormalities in raw semen were evaluated through a computer-assisted semen analysis system (Magavision®, Magapor).
Semen doses analysis
Ten CAI semen doses and 16 PCAI semen doses were collected monthly from each boar stud and sent to the laboratory for sperm concentration and volume determination (totalizing 3,833 semen doses). The volume was verified by weighing the semen dose content, and sperm concentration was determined using a hemocytometer chamber (Neubauer Improved, Optik Labor) after diluting 100 µL of semen dose in formalin solution (900 µL).
Microbiological analyses
Sample collection
For each ejaculate collected in each boar stud, five samples of raw semen, extended semen, and semen doses stored in the boar stud were collected monthly for microbiological analyses. Moreover, five samples of boar semen doses were collected at the destination farm. Water samples from boar studs were also collected monthly: one sample of unpurified water from the stud entrance, another sample of water submitted to the reverse osmosis process, and a further sample of water submitted to the reverse osmosis process and stored for 24 h at room temperature (~ 24 °C; stored water). Additionally, one sample of the extender freshly prepared was obtained. All samples were collected using sterile containers and stored at 2-8 °C until analysis.
Counting and identification of aerobic mesophiles
At the laboratory, samples were submitted to serial dilution. Microbiological analysis was carried out using the spread plate technique, in plate count agar (PCA) which was incubated for 48 h at 37 °C. The number of colonies forming units per mL (CFU mL1) was determined after 48 h incubation at 37 °C. Raw semen samples presenting > 2,000 CFU mL1were considered contaminated, as well as the extended semen, boar semen doses (stored in the boar stud or the destination farm), and extender when counting was ≥ 1 CFU mL1. For water submitted to the reverse osmosis process (stored or not), samples with ≥ 1 CFU mL1were classified as contaminated, while for unpurified water samples, contamination was considered when counting > 1,000 CFU mL1.
Isolated colonies were evaluated by biochemical testing. Gram-positive and Gram-negative bacteria were identified using 3 % potassium hydroxide (KOH) and cultured in Rugai-modified medium with lysine. Gram-positive bacteria were submitted to the catalase, coagulase, 6.5 % sodium chloride (NaCl) and bile-esculin tests.
Statistical analyses
Statistical analyses were conducted using SAS® software (SAS Institute Inc. Release 9.4). Noncompliance items were tested as potential risk factors for 13 response variables of interest. Eleven of these response variables were dichotomous and, therefore, evaluated through logistic regression models: 1) contamination in raw semen; 2) in extended semen; 3) in semen stored in the stud; 4) in semen stored at the farm of origination; 5) in unpurified water; 6) in water submitted to the reverse osmosis process; 7) in stored water; 8) in the extender; 9) occurrence of semen doses with more than 3.4 × 109sperm cells in 80 mL; 10) occurrence of ejaculates with more than 30 % sperm cells with morphological abnormalities; and 11) occurrence of ejaculates with sperm motility inferior to 70 %.
After checking for normality using the Shapiro-Wilk test, multiple linear regression was applied to evaluate the remaining two response variables (continuous variables): ejaculate volume (12) and the total number of sperm cells in ejaculates (13). For all responses (dichotomous or continuous), the period of analyses considered an interval of 60-days (30 days before and 30 days after applying each checklist). Differences were considered when p ≤ 0.05.
Thereafter, the boar studs were ranked according to scores corresponding to the frequency of identified compliance items related to semen quality and semen or water contamination: score one represented the maximum frequency while score 11 represented the minimum frequency. Subsequently, a median score was determined to rank each stud according to its frequency of compliance items.
Results
On average, the audited boar studs presented an inventory of 150 boars and a monthly production of 16,622 semen doses during the period evaluated (112.9 semen doses per boar per month), most of them being produced for PCAI (74 %). The total number of sperm cells in CAI semen doses was 3.2 ± 0.2 billion; however, 35 % of these semen doses had more than 3.5 billion sperm cells. For PCAI semen doses, the average total number of sperm cells was 1.9 ± 0.1 billion, with 62.1 % of them presenting more than 1.8 billion sperm cells. The coefficient of variation for total sperm number was similar for CAI and PCAI semen doses (Table 2; Figure 1).
– Frequency distribution of PCAI and CAI semen doses (n = 1,420 and 2,143, respectively) produced by 11 Brazilian boar studs audited by veterinary services over 24 months, according to their total number of sperm cells. PCAI = post-cervical artificial insemination (semen doses with 1.6 ± 0.3 billion cells; coefficient of variation = 14.9 %). CAI = cervical artificial insemination (semen doses with 3.3 ± 0.5 billion cells; coefficient of variation = 14.1 %).
A decrease in the volume of raw semen was associated with the seasonal increase in temperature; however, the parameter increased when the interval between semen collections was inadequate (≤ 2 days or > 7 days; Table 3; p < 0.01). Seasonal increase in temperatures were also related to a decrease in sperm concentration of raw semen (p = 0.03), which was also associated with the lack of height adjustment of the semen collection dummy (p < 0.01) and the lack of anti-slip rubber mat in the semen collection area (p = 0.03).
No risk factor was associated with a total sperm number > 1.8 billion in PCAI semen doses or ≥ 3.4 billion in CAI semen doses (p > 0.05). The odds of observing > 30 % of sperm morphological abnormalities in raw semen were 1.4 times greater when the laboratory equipment was poorly calibrated or monitored (p = 0.03), 1.5 times greater when boar housing was inadequate, and 1.7 times greater when semen was collected by a non-experienced technician or when the interval between semen collections was inadequate (p < 0.02). The odds of raw semen presenting sperm motility < 70 % was 1.7 greater when no anti-slip rubber mat in the semen collection area was used, no cleaning program for the automatic feeding system and bins was followed, or the interval between semen collections was inadequate (p < 0.01; Table 4).
The risk factors associated with semen contamination are shown in Table 5. The odds of contamination in raw semen were more than two times greater when there was no anti-slip rubber mat in the semen collection area or when boar prepuce was poorly cleaned. When boars were not adequately housed or when the seasonal temperature increased, the odds of raw semen contamination were at least 1.7 times greater (p < 0.03). For contamination of extended semen, the odds were at least eight times greater when non-disposable material was used for semen processing, when laboratory equipment was not adequately cleaned, and when the extender was contaminated (p < 0.01). Contamination odds in semen doses stored in the boar stud were at least four times greater (p < 0.01) when there was no regular change of reverse osmosis filters or when the herd presented an incidence of locomotor problems > 5 %.
For semen doses stored at the destination farm, the odds of contamination were 1.96 times greater when non-disposable materials were used for semen processing (p = 0.01), and more than two times greater when the laboratory equipment was not adequately cleaned (p = 0.03) or when the evaluation of semen motility was deficient (p = 0.01). In addition, the contamination odds of semen doses stored at the destination farm increased by 3.5 and 5.8 times when the extender was contaminated and the semen was collected by a non-experienced technician, respectively (p < 0.01). Seasonal temperature increases doubled the odds of contamination in the unpurified water (p = 0.02; Table 5).
The odds of contamination in water submitted to the reverse osmosis process were more than 4.8 times greater when the purification equipment was not cleaned and disinfected (p = 0.01). For water submitted to the reverse osmosis process and stored at room temperature for 24 h, the odds of contamination were 4.3 times greater when water submitted to the reverse osmosis process (but not stored) was contaminated and 6.9 times greater when the laboratory equipment was not adequately cleaned (p < 0.01). Inadequate cleaning of laboratory equipment was also associated with extender contamination, increasing the odds of extender contamination by almost five times (p = 0.02; Table 5). In the raw semen and water samples, 25 distinct microorganisms were isolated, with a higher frequency of Gram-negative bacteria (Table 6).
Comparing the sperm quality items among the boar studs (Table 7), more than 90 % compliance was observed for items related to reduced contamination in semen doses. Compliance higher than 90 % was also observed for items associated with sperm quality, such as frequency of raw semen with total sperm motility > 70 % or morphological abnormalities < 30 %, and frequency of semen doses (CAI or PCAI) containing the target total sperm number. On the other hand, lower compliance (≤ 65.5 %) was observed for items such as contamination of water submitted to the reverse osmosis process and contamination of raw semen. Overall, median scores indicating a higher frequency of compliance were observed in three boar studs (identified in Table 7 as boar studs ‘J’, ‘C’, and ‘G’; median scores: 3, 4, and 4; respectively). Additionally, three boar studs presented median scores indicating a lower frequency of compliance (boar studs identified in Table 7 as ‘E’, ‘D’ and ‘I’, with median scores 8, 9, and 10, respectively).
Discussion
Our results showed that indicators of semen quality (e.g., sperm motility, morphological abnormalities, and concentration in raw semen) were negatively influenced by several risk factors: poor calibration and maintenance of laboratory equipment; inadequate cleaning of the automatic feeding system and bins; semen collection by a non-experienced technician; no adjustments on dummy according to the boar’s height; and an inadequate interval between collections (≤ 2 days or > 7 days). Considering a two-day interval as a minimum period between consecutive semen collections, it should not be excessively shortened in periods of increased semen demand to prevent the reduction in the ejaculate’s volume and impairment in semen quality, since a short transit of the semen through the epididymis would jeopardize sperm maturation (Pruneda et al., 2005Pruneda A, Pinart E, Briz MD, Sancho S, Garcia-Gil N, Badia E, et al. 2005. Effects of a high semen-collection frequency on the quality of sperm from ejaculates and from six epididymal regions in boars. Theriogenology 63: 2219-2232. https://doi.org/10.1016/j.theriogenology.2004.10.009
https://doi.org/10.1016/j.theriogenology...
).
In the present study, approximately 74 % of the semen doses produced in studs evaluated were for post-cervical AI (45 mL), containing an average of 1.9 billion sperm cells. The PCAI shows a wide-spread commercial use for sows, mainly in South America (García-Vázquez et al., 2019García-Vázquez FA, Mellagi APG, Ulguim RR, Hernández-Caravaca I, Llamas-López PJ, Bortolozzo FP. 2019. Post-cervical artificial insemination in porcine: The technique that came to stay. Theriogenology 129: 37-45. https://doi.org/10.1016/j.theriogenology.2019.02.004
https://doi.org/10.1016/j.theriogenology...
), and is currently being performed with semen doses containing 1.0-2.0 billion sperm cells in 40-50 mL (Bortolozzo et al., 2015 Bortolozzo FP , Menegat MB , Mellagi APG , Bernardi ML , Wentz I . 2015. New artificial insemination technologies for swine. Reproduction in Domestic Animals 50: 80-84. https://doi.org/10.1111/rda.12544
https://doi.org/10.1111/rda.12544...
; Waberski et al., 2019Waberski D, Riesenbeck A, Schulze M, Weitze KF, Johnson L. 2019. Application of preserved boar semen for artificial insemination: Past, present and future challenges. Theriogenology 137: 2-7. https://doi.org/10.1016/j.theriogenology.2019.05.030
https://doi.org/10.1016/j.theriogenology...
). The use of semen doses with 2.5-4 billion sperm cells in 70-100 mL have been mostly used for CAI (Soriano-Úbeda et al., 2013Soriano-Úbeda C, Matás C, García-Vázquez FA. 2013. An overview of swine artificial insemination: retrospective, current and prospective aspects. Journal of Experimental and Applied Animal Sciences 1: 67-97. http://dx.doi.org/10.20454/jeaas.2013.709
http://dx.doi.org/10.20454/jeaas.2013.70...
; Bortolozzo et al., 2015 Bortolozzo FP , Menegat MB , Mellagi APG , Bernardi ML , Wentz I . 2015. New artificial insemination technologies for swine. Reproduction in Domestic Animals 50: 80-84. https://doi.org/10.1111/rda.12544
https://doi.org/10.1111/rda.12544...
; Knox, 2016Knox RV, 2016. Artificial insemination in pigs today. Theriogenology 85: 83-93. https://doi.org/10.1016/j.theriogenology.2015.07.009
https://doi.org/10.1016/j.theriogenology...
; Roca et al., 2016Roca J, Parrilla I, Bolarin A, Martinez EA, Rodriguez-Martinez H. 2016. Will AI in pigs become more efficient? Theriogenology 86: 187-193. http://dx.doi.org/10.1016/j.theriogenology.2015.11.026
http://dx.doi.org/10.1016/j.theriogenolo...
), and the average value observed in this investigation for CAI semen doses (80 mL) was 3.3 billion sperm cells. Overall, it is essential to highlight that both PCAI and CAI semen doses presented a sperm concentration (~ 40 million mL1) under the limit currently recommended (~ 60 million mL1) to avoid low sperm motility over the storage period (≤ 70 %; Quirino et al., 2023Quirino M, Rosa GT, Christ TS, Valadares WR, Ulguim RR, Bernardi ML, et al. 2023. Estimation of sperm concentration limits to produce intrauterine insemination doses in swine. Reproduction in Domestic Animals 58: 785-792. https://doi.org/10.1111/rda.14351
https://doi.org/10.1111/rda.14351...
). Our data also showed some dispersion beyond the average values of total sperm number, which was observed for all studs evaluated, regardless of the type of semen dose, as indicated by coefficients of variation of 14-15 %. This information must be highlighted since this parameter is associated with semen dose quality and with the optimization of ejaculate use.
It has already been observed that high levels of bacterial contamination in boar semen are associated with sperm agglutination, damaged acrosomes, poor sperm motility, reduced shelf life of the extended semen product (Wolff et al., 1993Wolff H, Panhans A, Stolz W, Meurer M. 1993. Adherence of Escherichia coli to sperm: a mannose mediated phenomenon leading to agglutination of sperm and E. coli. Fertility and Sterility 60: 154-158. https://doi.org/10.1016/S0015-0282 (16)56054-3
https://doi.org/10.1016/S0015-0282 (16)5...
; Auroux et al., 1991Auroux MR, Jacques L, Mathieu D, Auer J. 1991. Is the sperm bacterial ratio a determining factor in impairment of sperm motility: an in-vitro study in man with Escherichia coli. International Journal of Andrology 14: 264-270. https://doi.org/10.1111/j.1365-2605.1991.tb01091.x
https://doi.org/10.1111/j.1365-2605.1991...
; Úbeda et al., 2013Úbeda JL, Ausejo R, Dahmani Y, Falceto MV, Usan A, Malo C, et al. 2013. Adverse effects of members of the Enterobacteriaceae family on boar sperm quality. Theriogenology 80: 565-570. https://doi.org/10.1016/j.theriogenology.2013.05.022
https://doi.org/10.1016/j.theriogenology...
; Prieto-Martínez et al., 2014Prieto-Martínez N, Bussalleu E, Garcia-Bonavila E, Bonet S, Yeste M. 2014. Effects of Enterobacter cloacae on boar sperm quality during liquid storage at 17 °C. Animal Reproduction Science 148: 72-82. https://doi.org/10.1016/j.anireprosci.2014.05.008
https://doi.org/10.1016/j.anireprosci.20...
), and detrimental effects on reproductive performance (Maroto-Martín et al., 2010Maroto-Martín LO, Munõz EC, De Cupere F, Van Driessche E, Echemendia-Blanco D, Rodriguez JMM, et al. 2010. Bacterial contamination of boar semen affects the litter size. Animal Reproduction Science 120: 95-104. https://doi.org/10.1016/j.anireprosci.2010.03.008
https://doi.org/10.1016/j.anireprosci.20...
; Úbeda et al., 2013Úbeda JL, Ausejo R, Dahmani Y, Falceto MV, Usan A, Malo C, et al. 2013. Adverse effects of members of the Enterobacteriaceae family on boar sperm quality. Theriogenology 80: 565-570. https://doi.org/10.1016/j.theriogenology.2013.05.022
https://doi.org/10.1016/j.theriogenology...
; Sepulveda et al., 2014Sepulveda L, Bussalleu E, Yeste M, Bonet S. 2014. Effects of different concentrations of Pseudomonas aeruginosa on boar sperm quality. Animal Reproduction Science 150: 96-106. https://doi.org/10.1016/j.anireprosci.2014.09.001
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). This scenario may be aggravated by the resistance of microorganisms isolated in semen samples to commonly used antimicrobials, as reported for boar (Schulze et al., 2015Schulze M, Ammon C, Rüdiger K, Jung M, Grobbel M. 2015. Analysis of hygienic critical control points in boar semen production. Theriogenology 83: 430-437. https://doi.org/10.1016/j.theriogenology.2014.10.004
https://doi.org/10.1016/j.theriogenology...
; Costinar et al., 2022 Costinar L , Herman V , Pitoiu E , Iancu I , Degi J , Hulea A , et al . 2022. Boar semen contamination: identification of Gram-negative bacteria and antimicrobial resistance profile. Animals 12: 43. https://doi.org/10.3390/ani12010043
https://doi.org/10.3390/ani12010043...
) and bull semen (Goularte et al., 2020 Goularte KL , Voloski FLS , Redú JFM , Ferreira CER , Vieira AD , Duval EH , et al . 2020. Antibiotic resistance in microorganisms isolated in a bull semen stud. Reproduction in Domestic Animals 55: 318-324. https://doi.org/10.1111/rda.13621
https://doi.org/10.1111/rda.13621...
). Our data showed that a wide variety of microorganisms were isolated from raw semen samples, as has already been reported in other studies (Althouse et al., 2008Althouse GC, Pierdon MS, Lu KG. 2008. Thermotemporal dynamics of contaminant bacteria and antimicrobials in extended porcine semen. Theriogenology 70: 1317-1323. https://doi.org/10.1016/j.theriogenology.2008.07.010
https://doi.org/10.1016/j.theriogenology...
; Maroto-Martín et al., 2010Maroto-Martín LO, Munõz EC, De Cupere F, Van Driessche E, Echemendia-Blanco D, Rodriguez JMM, et al. 2010. Bacterial contamination of boar semen affects the litter size. Animal Reproduction Science 120: 95-104. https://doi.org/10.1016/j.anireprosci.2010.03.008
https://doi.org/10.1016/j.anireprosci.20...
; Kuster and Althouse, 2016Kuster CE, Althouse GC. 2016. The impact of bacteriospermia on boar sperm storage and reproductive performance. Theriogenology 85: 21-26. https://doi.org/10.1016/j.theriogenology.2015.09.049
https://doi.org/10.1016/j.theriogenology...
), which confirms the relevant prevalence of Gram-negative bacteria in raw semen (Úbeda et al., 2013Úbeda JL, Ausejo R, Dahmani Y, Falceto MV, Usan A, Malo C, et al. 2013. Adverse effects of members of the Enterobacteriaceae family on boar sperm quality. Theriogenology 80: 565-570. https://doi.org/10.1016/j.theriogenology.2013.05.022
https://doi.org/10.1016/j.theriogenology...
; Costinar et al., 2022 Costinar L , Herman V , Pitoiu E , Iancu I , Degi J , Hulea A , et al . 2022. Boar semen contamination: identification of Gram-negative bacteria and antimicrobial resistance profile. Animals 12: 43. https://doi.org/10.3390/ani12010043
https://doi.org/10.3390/ani12010043...
). As a collection of fully sterile ejaculates is nearly unfeasible (Schulze et al., 2015Schulze M, Ammon C, Rüdiger K, Jung M, Grobbel M. 2015. Analysis of hygienic critical control points in boar semen production. Theriogenology 83: 430-437. https://doi.org/10.1016/j.theriogenology.2014.10.004
https://doi.org/10.1016/j.theriogenology...
), some level of semen contamination is expected before processing. For this reason, in the present study, raw semen was considered contaminated when containing more than 2,000 CFU mL1. However, a previous study reported that boar sperm quality would be impaired in ejaculates containing more than 1,000 CFU mL1 (Goldberg et al., 2013Goldberg AMG, Argenti LE, Faccin JE, Linck J, Santi M, Bernardi ML, et al. 2013. Risk factors for bacterial contamination during boar semen collection. Research in Veterinary Science 95: 362-367. https://doi.org/10.1016/j.rvsc.2013.06.022
https://doi.org/10.1016/j.rvsc.2013.06.0...
), which emphasizes that determining the tolerable contamination levels in raw boar semen is a complex task.
It may be expected that the risk factors for contamination in raw semen would be related to the collection process. The prepuce is a relevant source of contamination of ejaculates if basic hygiene procedures (e.g., dry cleaning of the prepuce before semen collection) are neglected (Goldberg et al., 2013Goldberg AMG, Argenti LE, Faccin JE, Linck J, Santi M, Bernardi ML, et al. 2013. Risk factors for bacterial contamination during boar semen collection. Research in Veterinary Science 95: 362-367. https://doi.org/10.1016/j.rvsc.2013.06.022
https://doi.org/10.1016/j.rvsc.2013.06.0...
), which was confirmed in the present study by contamination odds that were at least 2.6 times greater when hygiene procedures were not properly followed. Additionally, the odds of contamination in raw semen increased when there was inadequate boar housing and no anti-slip rubber mat in the semen collection area. Housing factors such as barn dimensions, drainage of manure, and humidity levels may influence the accumulation of dirt in the ventral abdomen, thereby affecting the chances of semen contamination during its collection (Althouse et al., 2000Althouse GC, Kuster CE, Clark SG, Weisiger RM. 2000. Field investigations of bacterial contaminants and their effects on extended porcine semen. Theriogenology 53: 1167-1176. https://doi.org/10.1016/S0093-691X (00)00261-2
https://doi.org/10.1016/S0093-691X (00)0...
). Moreover, inappropriate housing can increase the occurrence of locomotor problems, which increases the odds of contamination in the semen doses stored at the stud. Locomotor problems affect the capacity of boars to sustain themselves adequately during semen collection, consequently increasing the chances of semen contamination. Thus, boar housing conditions must be constantly monitored to prevent inadequate welfare conditions for boars. The absence of a non-slip rubber mat may result in a slippery floor in the semen collection area, making it difficult for the boars to sustain an adequate position during semen collection. Indeed, this risk factor was not only associated with higher contamination odds in raw semen but was also related to increased odds of occurrence of ejaculates with less than 70 % sperm motility.
The odds of contamination in raw semen also increased with seasonal increases in temperature, which were also associated with adverse effects on the volume and sperm concentration of raw semen, as well as water contamination. Although heat-stressed boars may have impaired semen quality and decreased fertility (Peña Jr. et al., 2019), only marginal effects of seasonal temperature increase on boar sperm quality in subtropical areas such as have been reported (Argenti et al., 2018 Argenti LE , Parmeggiani BS , Leipnitz G , Weber A , Pereira GR , Bustamante-Filho IC . 2018. Effects of season on boar semen parameters and antioxidant enzymes in the south subtropical region in Brazil. Andrologia 50: e12951. https://doi.org/10.1111/and.12951
https://doi.org/10.1111/and.12951...
). However, seasonal fluctuations in semen contamination impairing semen quality were reported, with multifactorial interactions with the extender quality, the prevalence of contaminant microorganisms, and the efficiency of antimicrobials (Althouse et al., 2008Althouse GC, Pierdon MS, Lu KG. 2008. Thermotemporal dynamics of contaminant bacteria and antimicrobials in extended porcine semen. Theriogenology 70: 1317-1323. https://doi.org/10.1016/j.theriogenology.2008.07.010
https://doi.org/10.1016/j.theriogenology...
). All boar studs evaluated in this study presented temperature control through air conditioners; however, it did not prevent the potential effects of seasonal temperature increasing on the quality of the ejaculates. It suggests that adjustments in temperature control systems inside the studs throughout the year may be required to compensate for seasonal fluctuations in environmental temperatures.
As semen contamination after collection and processing is supposed to be minimal in commercial studs with strict biosecurity, extended semen was considered contaminated when containing ≥ 1 CFU mL1. The risk factors for contamination in extended semen were related to neglected laboratory procedures, such as the use of non-disposable material and the poor cleaning of equipment, as has been reported in other studies (Schulze, et al., 2015; Nitsche-Melkus et al., 2020Nitsche-Melkus E, Bortfeldt R, Jung M, Schulze M. 2020. Impact of hygiene on bacterial contamination in extended boar semen: an eight-year retrospective study of 28 European Al centers. Theriogenology 146: 133-139. https://doi.org/10.1016/j.theriogenology.2019.11.031
https://doi.org/10.1016/j.theriogenology...
). These risk factors were associated with semen dose contamination at the destination farm. In addition, the inadequate cleaning of laboratory equipment was identified as a risk factor for extender contamination, which was also a risk for contamination of extended semen and semen doses stored at the destination farm. These findings emphasize that procedures related to the semen processing routine at the boar studs influence semen quality at subsequent stages. As most microorganisms isolated in the present study can be considered opportunistic, their presence in the semen and in the extender may result from an inadequate cleaning process of laboratory material, leading to the formation of biofilm. (Waberski, 2019; Costinar et al., 2022 Costinar L , Herman V , Pitoiu E , Iancu I , Degi J , Hulea A , et al . 2022. Boar semen contamination: identification of Gram-negative bacteria and antimicrobial resistance profile. Animals 12: 43. https://doi.org/10.3390/ani12010043
https://doi.org/10.3390/ani12010043...
).
As has been previously reported, failures in the water purification process and manipulation during the semen processing result in water contamination (Úbeda et al., 2013Úbeda JL, Ausejo R, Dahmani Y, Falceto MV, Usan A, Malo C, et al. 2013. Adverse effects of members of the Enterobacteriaceae family on boar sperm quality. Theriogenology 80: 565-570. https://doi.org/10.1016/j.theriogenology.2013.05.022
https://doi.org/10.1016/j.theriogenology...
). Although the odds of contamination in unpurified water increased with high seasonal temperatures, purification processes could mitigate such contamination. Nonetheless, the odds of contamination in stored water were increased when the process of cleaning and disinfecting the purification system or cleaning the laboratory equipment were inefficient, leading to higher odds of water contamination even after the reverse osmosis process. Our results identified associations between water contamination and semen contamination, as the lack of a scheduled change of reverse osmosis filters was a risk factor for contamination in the semen stored at the stud. Those findings may reflect that the water supplied to the evaluated boar studs had not been treated with chloride since it was mostly from natural and artesian wells. Therefore, constant maintenance and cleaning of the equipment used for water purification is mandatory. It is also important to mention that, in this investigation, the composition of some materials, such as semen packages, was not assessed. Nevertheless, this approach can be considered in quality control programs since the contact of sperm cells with toxic compounds can result in additional detrimental effects on subsequent fertility after AI, even when adverse effects on semen quality are not evident (Nerin et al., 2014 Nerin C , Ubeda JL , Alfaro P , Dahmani Y , Aznar M , Canellas E , et al . 2014. Compounds from multilayer plastic bags cause reproductive failures in artificial insemination. Scientific Reports 4: 4913. https://doi.org/10.1038/srep04913
https://doi.org/10.1038/srep04913...
; Schulze et al., 2020 Schulze M , Schröter F , Jung M , Jakop U . 2020. Evaluation of a panel of spermatological methods for assessing reprotoxic compounds in multilayer semen plastic bags. Scientific Reports 10: 22258. https://doi.org/10.1038/s41598-020-79415-7
https://doi.org/10.1038/s41598-020-79415...
).
The studs evaluated in this study represent nearly 20 % of Brazil’s boar inventory and 15 % of the semen doses currently produced in the Brazilian swine industry. The quality control comparison across studs indicated that studs E, D, and I presented greater noncompliance frequencies, especially for items related to semen quality. However, Stud E ranked particularly worse in items related to semen contamination. Furthermore, studs D and E produced the lowest number of semen doses per boar per month. On the other hand, studs J, C, and G presented greater compliance frequencies. Although studs J and G had the lowest boar inventories (< 100 boars) and were among the studs with lower monthly production of semen doses, the semen produced in such studs was likely high-quality. Thus, as all studs evaluated were periodically audited by the same veterinary service, stud J, with a median score equal to three, would be a candidate as a reference to benchmark the remaining studs. However, this boar stud would still need to improve a noncompliance issue for a fundamental item: contamination of water submitted to the reverse osmosis process. Additionally, stud C could also be considered a reference since it achieved a similar median score (4) and presented the greatest production of semen doses/boar/month, likely due to its large boar inventory.
The quality control audits in 11 Brazilian boar studs over 24 months revealed that factors mainly related to semen collection were associated with increased odds of reduced semen quality. In contrast, the risk of water and semen contamination was increased by deficient cleaning and disinfection of equipment. Given these data, constant monitoring, appropriate hygiene of the facilities and equipment, and periodical staff training can be highlighted as non-negotiable points for boar studs. Out of all the boar studs evaluated, three could qualify as potential benchmarks due to their higher frequency of compliance with the checklist items. Nevertheless, we do recommend implementing the quality control approach in a higher number of boar studs in Brazil, making possible further characterization and monitoring of the semen process in the Brazilian swine industry, consequently guaranteeing the production of high-quality boar semen doses.
Acknowledgments
The authors are grateful to Bretanha Suínos (Brasil), Embrapa Suínos e Aves, Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq), Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES), and Fundação de Amparo à Pesquisa e Inovação do Estado de Santa Catarina (FAPESC).
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Publication Dates
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Publication in this collection
22 July 2024 -
Date of issue
2024
History
-
Received
05 July 2023 -
Accepted
12 Nov 2023