RESUMO

While sperm migrate within the reproductive tract of cows experiencing negative energy balance (NEB), they come into contact with elevated concentrations of non-esterified fatty acids (NEFA). For this reason, this study aimed to investigate the effects of three different NEFA - palmitic acid (PA), stearic acid (SA), and oleic acid (OA) - on bovine sperm motility, kinetic parameters, oxidative status, and morphology. Frozen thawed semen samples from Bos taurus bulls were incubated with varying concentrations of each fatty acid, and the sperm's characteristics were analysed at different time points. Computer-Assisted Sperm Analysis (CASA) was employed to assess sperm motility and kinetic parameters. Concurrently, the production of the reactive oxygen species (ROS) and total antioxidant capacity were measured to determine the oxidative status. Additionally, sperm morphology was evaluated. In Experiment 1, different concentrations of PA did not show significant effects on total motility, progressive motility, or any kinetic parameters analysed. Similarly, PA did not have a significant impact on the oxidative status or sperm morphology. In Experiment 2, SA at various concentrations did not lead to significant changes in total motility, progressive motility, or any kinetic parameters evaluated. Furthermore, SA did not affect oxidative status or sperm morphology. In Experiment 3, the concentrations of OA used did not result in significant changes in total motility, progressive motility, or any kinetic parameters studied. Likewise, OA did not induce any alterations in oxidative status or sperm morphology. Overall, the results from all three experiments indicate that PA, SA and OA, at the in vitro conditions and tested concentrations, do not exert detrimental effects on bovine sperm function and morphology. These results provide insights that contribute to our understanding of how fatty acids can impact the reduction of fertility rates in cows facing NEB. This, in turn, lays the foundation for additional critical investigations in this area. Further studies are necessary to validate these findings in vivo.

Assuntos

RESUMO

Veterinary drugs are potential environmental pollutants that interfere with male reproductive function. Infertility has increased, and it is known that environmental toxins contribute to declining sperm parameters. Amitraz {N,N-[(methylamino) dimeth-ylidyne] di-2,4-xylidine} (AMZ) is a formamidine pesticide widely used as an insecticide and an acaricide. The aim of this study was to evaluate the toxicity of AMZ in bovine sperm. Three experiments using frozen-thawed bovine semen incubated with AMZ for 2 h were carried out. Negative and solvent (dimethyl sulfoxide) controls were run simultaneously with treatments. In experiment 1, the AMZ concentrations used were 10, 15 and 25 µg AMZ/ml and the sperm parameters evaluated were viability, mitochondrial activity, acrosomal status, functional membrane integrity and apoptosis. In experiments 2 and 3, 25 µg AMZ/ml was used to evaluate fertilizing capacity, embryo development and blastocyst DNA damage. In experiment 1, 25 µg AMZ/ml decreased sperm viability (P = 0.01), reduced mitochondrial activity (P = 0.03) and induced apoptosis (P < 0.01). Also, 15 and 25 µg AMZ/ml affected functional membrane integrity (P < 0.01). In experiment 2, AMZ did not alter sperm-zona binding (P = 0.40) and pronucleus formation (P = 0.36). In experiment 3, 25 µg AMZ/ml decreased the rate of embryo development (P < 0.01) and increased apoptosis (P = 0.03). These results suggest that AMZ induced alterations in bovine sperm, probably affecting male fertility at concentrations that could be present in the environment.

Assuntos

RESUMO

The acetic acid-urea polyacrylamide gel electrophoresis system could separate very similar basic proteins on differences in size and effective charge. This system has been used for many years to analyse histones and their post-translational modifications and widely used in the study of mammal protamines. Two types of protamine have been described, the protamine 1 (P1) and the protamine 2 (P2) family members, which are synthetized by PRM1 and PRM2 genes. The ratio of P1 and P2 is important for predicting fertility in humans and mice. Therefore, the quantification of protamines is a fundamental step in order to establish the ratio between P1 and P2 in these species. In other mammals, studies linking sperm protamination and the protamine ratio with fertility are increasing. So, the use of an effective technique to separate and quantify protamines is important to study sperm P1/P2 ratio. Therefore, this article describes in detail a feasible and useful procedure to isolate bovine sperm protamines, to perform pre-electrophoresis with PEG solution and finally to carry out acid-urea polyacrylamide gel electrophoresis in reverse polarity. This technique allows a clear separation and efficient detection of bovine sperm protamines.

Assuntos

RESUMO

RESUMEN: En el semen criopreservado, los procesos de congelación/descongelación y posterior manipulación, dañan las células espermáticas provocando disminución de la capacidad fecundante de los espermatozoides descongelados. Estos procesos han sido asociados con el estado de estrés oxidativo (EO) inducido por altos niveles de especies reactivas de oxígeno (EROS), causando daño a la función y estructura espermática. Los espermatozoides descongelados pueden ser protegidos de este daño, con la adición de antioxidantes (AO) al medio de incubación. El fruto de Calafate (Berberis microphylla G. Forst.) posee una alta capacidad antioxidante, lo que hace interesante investigar el efecto de sus componentes antioxidantes en estos procesos biotecnológicos especialmente postdescongelación. El objetivo de este estudio fue determinar el efecto de la suplementación de extracto liofilizado de fruto de Calafate (ELC), sobre la calidad espermática post-descongelación. Previamente se caracterizó el ELC, determinando la actividad antioxidante y metabolitos como fenoles y antocianinas; posteriormente, espermatozoides de bovino descongelados fueron incubados en un medio base suplementado con diferentes concentraciones de ELC. Post-incubación se evaluó la motilidad progresiva; la viabilidad e integridad de la membrana plasmática (SYBR14- PI) y acrosomal (FITC-PNA/PI) y la peroxidación lipídica (BODIPY) por citometría de flujo. La caracterización de ELC demostró que tanto la actividad antioxidante como los fenoles y antocianinas incrementan concomitante con el aumento de la concentración de ELC. La adición de ELC al medio de incubación, dependiendo de la concentración y tiempo de incubación, sería eficaz en proteger la motilidad, viabilidad e integridad de la membrana plasmática y disminuir la lipoperoxidación en los espermatozoides de bovino descongelados.

SUMMARY: In cryopreserved semen, the freezing/thawing process following of manipulation, damage the sperm cell, decreasing the fertilizing capacity of the thawed sperm; being one of the main factors of this damage the oxidative stress. The sperm once thawed can be protected from this damage, with the addition of antioxidants to the incubation medium. The Calafate fruit (Berberis microphylla G. Forst.) has a high antioxidant capacity, making it an interesting resource for investigating the effect of its antioxidant components on biotechnological processes. The objective of this study was to determine the effect of supplementation of Calafate fruit lyophilized extract (ELC) on sperm quality. The lyophilized extract of the Calafate fruit was characterized, determining the antioxidant activity and metabolites such as phenols and anthocyanins; subsequently, thawed bovine sperm were incubated in a medium supplemented with different concentrations of ELC. Post-incubation, progressive motility was evaluated. By flow cytometry, the viability and integrity of the plasma (SYBR14-PI), and acrosomal (FITC-PNA / PI), as well as lipid peroxidation (BODIPY), was determined. The characterization of Calafate fruits lyophilized extract indicated that antioxidant activity, phenols and anthocyanins increased concomitantly with the increase of dose extract used. The addition of ELC to the incubation medium, depending on the concentration and incubation time, would be effective to protect motility, viability and integrity of the plasma membrane and decreased lipid peroxidation in thawed bovine sperm.

Assuntos

RESUMO

SummaryThe cryopreservation of epididymal sperm is an important technique that allows genetic material to be preserved, even post mortem. However, cryopreservation leads to increased oxidative stress and impaired sperm viability. Polyunsaturated fatty acid (PUFA) supplementation may improve certain sperm characteristics, but it also makes sperm more susceptible to oxidative stress, therefore adding antioxidants that counteract oxidative stress has become an option. In this context, this study aimed to evaluate the effect of the interaction between docosahexaenoic acid (DHA) and antioxidants on the quality after the cryopreservation of epididymal bull sperm. Twenty epididymides were collected after slaughter, and epididymal sperm was cryopreserved with bovine extender supplemented with docosahexaenoic acid (DHA), glutathione peroxidase (GPx) and superoxide dismutase (SOD). We verified an improvement in motility in the group that was treated only with DHA 5 µM and a concentration-dependent effect on susceptibility to lipid peroxidation that was associated with DHA concentration (1 µM, 5 µM or 10 µM). Moreover, treatment with DHA (5 µM) and SOD (20 IU/ml) resulted in higher sperm motility. Thus, the association between DHA (5 µM) and SOD (20 IU/ml) appears to be an option for increased epididymal sperm features in bulls.

Assuntos

RESUMO

This study assesses the effect of bovine sperm (obtained from three bulls) separation using density gradients (Percoll and BoviPure) and Swim-up on sperm function and gene expression. Sperm evaluations included the plasma membrane integrity (SYBR14/PI), acrosomal integrity (PNA-FITC/PI), oxidative stress (ROS; CH2FDDA), DNA fragmentation (TUNEL assay) and mitochondrial membrane potential (ΔYm; TMRM) using flow cytometry. Sperm motility was evaluated by computer-assisted sperm analysis (CASA) and gene expression using RT-qPCR. The results showed that separation by Percoll achieves a higher proportion of sperm with intact plasma and acrosomal membranes (89.8 and 87.5%, respectively) than the unseparated control (70.3 and 62.4%, respectively), as well as by Swim-up (74.9 and 63.3%, respectively) and BoviPure (83.3 and 80.4%, respectively). No differences were observed in the proportion of spermatozoa with high ΔΨm between Percoll and BoviPure (84.3% and 83.5%, respectively), which were higher than Swim-up and the unseparated control (72.8% and 43.8%, respectively). The ROS levels were higher in the spermatozoa separated by Percoll and no differences were observed in the sperm DNA integrity between all groups. The motility analysis showed that the separation methods improve (p<0.05) total and progressive motility compared to the control, with Percoll proving the most efficient in this regard. Finally, the gene expression analysis of leptin (LEP), aromatase cytochrome P450 (CYP19) and protamine I (PRM1), after validation of 6 reference genes, showed no differences between groups. In conclusion, bovine sperm separation using density gradient improves the parameters of motility and sperm function without affecting the gene expression.

Assuntos

RESUMO

O objetivo deste estudo foi comparar a eficiência do sistema automatizado (curva de resfriamento controlada eletronicamente) de congelação de sêmen bovino versus o sistema convencional (curva não controlada) por meio dos parâmetros de qualidade e viabilidade espermática no período pós-descongelação. O sêmen de quatro touros azebuados adultos foram criopreservados simultaneamente em meio tris, gema e glicerol 7%. A avaliação computadorizada do sêmen descongelado detectou os seguintes parâmetros: MP 56,50±22,25%; VAP 34,77±4,25µm/s; VSL 28,17±4,25 µm/s; VCL 58,45±6,85µm/s; STR 82,00±2,31%; LIN 49,50±3,32%, para o sistema automatizado e MP. 57,00±13,11%; VAP 25,75±1,66µm/s; VSL 23,32±1,99µm/s; VCL 63,32±1,79µm/s; STR 82,25±3,59µm/s; LIN 50,00±4,97µm/s para o sistema convencional. Os valores médios das avaliações de integridade de membrana plasmática e integridade acrossomal foram de 54,72±12,55% e 36,13±22,20% para o sistema automatizado e 53,22±13,22% e 47,26±5,74% para o sistema convencional, respectivamente. Com os parâmetros avaliados foi possível identificar que não houve diferença estatística entre os sistemas de criopreservação. Desta forma, a escolha do método de criopreservação do sêmen bovino para utilização direta na propriedade fica a critério do técnico responsável, que deverá se basear na realidade de cada propriedade. Para tanto, sempre se deve considerar que o sistema convencional pode trazer mais variações que o sistema automatizado que, apesar do custo do equipamento, pode garantir repetibilidade nos resultados e consequente qualidade do sêmen bovino criopreservado.

The objective of this study was to compare the efficiency of bovine semen cryopreservation using the controlledrate freezing machine versus the conventional method (uncontrolled curve) by the parameters of sperm quality and viability in post-thaw period. Semen from four adult crossbreed bulls was cryopreserved in Tris-yolk-glycerol medium. The computer assisted analysis of thawed semen detected the following results: PM 56.50±22.25%; VAP 34.77±4.25µm/s; VSL 28.17±4.25µm/s; VCL 58.45±6.85µm/s; STR 82.00±2.31%; LIN 49.50±3.32%, to automated system and PM 57.00±13.11%; VAP 25.75±1.66µm/s; VSL 23.32±1.99µm/s; VCL 63.32±1.79µm/s; STR 82.25±3.59µm/s; LIN 50.00±4.97µm/s to conventional cryopreservation system. The results of plasma membrane and acrosome integrity evaluation were 54.7±12.55% and 36.13±22.20% for the automated system and 53.22±13.22% and 47.26±5.74% for the conventional system, respectively. The parameters evaluated demonstrated that there was no statistical difference between the cryopreservation systems. Thus, the choice of the bovine semen cryopreservation method to be used on a farm is a responsibility of the technician, and should be based on the reality of each farm. Therefore, it is always necessary to consider that the conventional system of bovine semen cryopreservation can vary more than the automated system, which, despite the cost of the equipment, can ensure repeatability of the results and consequent quality of cryopreserved bovine semen.

Assuntos

RESUMO

O objetivo deste estudo foi comparar a eficiência do sistema automatizado (curva de resfriamento controlada eletronicamente) de congelação de sêmen bovino versus o sistema convencional (curva não controlada) por meio dos parâmetros de qualidade e viabilidade espermática no período pós-descongelação. O sêmen de quatro touros azebuados adultos foram criopreservados simultaneamente em meio tris, gema e glicerol 7%. A avaliação computadorizada do sêmen descongelado detectou os seguintes parâmetros: MP 56,50±22,25%; VAP 34,77±4,25µm/s; VSL 28,17±4,25 µm/s; VCL 58,45±6,85µm/s; STR 82,00±2,31%; LIN 49,50±3,32%, para o sistema automatizado e MP. 57,00±13,11%; VAP 25,75±1,66µm/s; VSL 23,32±1,99µm/s; VCL 63,32±1,79µm/s; STR 82,25±3,59µm/s; LIN 50,00±4,97µm/s para o sistema convencional. Os valores médios das avaliações de integridade de membrana plasmática e integridade acrossomal foram de 54,72±12,55% e 36,13±22,20% para o sistema automatizado e 53,22±13,22% e 47,26±5,74% para o sistema convencional, respectivamente. Com os parâmetros avaliados foi possível identificar que não houve diferença estatística entre os sistemas de criopreservação. Desta forma, a escolha do método de criopreservação do sêmen bovino para utilização direta na propriedade fica a critério do técnico responsável, que deverá se basear na realidade de cada propriedade. Para tanto, sempre se deve considerar que o sistema convencional pode trazer mais variações que o sistema automatizado que, apesar do custo do equipamento, pode garantir repetibilidade nos resultados e consequente qualidade do sêmen bovino criopreservado.(AU)

The objective of this study was to compare the efficiency of bovine semen cryopreservation using the controlledrate freezing machine versus the conventional method (uncontrolled curve) by the parameters of sperm quality and viability in post-thaw period. Semen from four adult crossbreed bulls was cryopreserved in Tris-yolk-glycerol medium. The computer assisted analysis of thawed semen detected the following results: PM 56.50±22.25%; VAP 34.77±4.25µm/s; VSL 28.17±4.25µm/s; VCL 58.45±6.85µm/s; STR 82.00±2.31%; LIN 49.50±3.32%, to automated system and PM 57.00±13.11%; VAP 25.75±1.66µm/s; VSL 23.32±1.99µm/s; VCL 63.32±1.79µm/s; STR 82.25±3.59µm/s; LIN 50.00±4.97µm/s to conventional cryopreservation system. The results of plasma membrane and acrosome integrity evaluation were 54.7±12.55% and 36.13±22.20% for the automated system and 53.22±13.22% and 47.26±5.74% for the conventional system, respectively. The parameters evaluated demonstrated that there was no statistical difference between the cryopreservation systems. Thus, the choice of the bovine semen cryopreservation method to be used on a farm is a responsibility of the technician, and should be based on the reality of each farm. Therefore, it is always necessary to consider that the conventional system of bovine semen cryopreservation can vary more than the automated system, which, despite the cost of the equipment, can ensure repeatability of the results and consequent quality of cryopreserved bovine semen.(AU)

Assuntos

RESUMO

The objective of this study was to compare the efficiency of bovine semen cryopreservation using the controlled-rate freezing machine versus the conventional method (uncontrolled curve) by the parameters of sperm quality and viability in post-thaw period. Semen from four adult crossbreed bulls was cryopreserved in Tris-yolk-glycerol medium. The computer assisted analysis of thawed semen detected the following results: PM 56.50±22.25%; VAP 34.77±4.25µm/s; VSL 28.17±4.25µm/s; VCL 58.45±6.85µm/s; STR 82.00±2.31%; LIN 49.50±3.32%, to automated system and PM 57.00±13.11%; VAP 25.75±1.66µm/s; VSL 23.32±1.99µm/s; VCL 63.32±1.79µm/s; STR 82.25±3.59µm/s; LIN 50.00±4.97µm/s to conventional cryopreservation system. The results of plasma membrane and acrosome integrity evaluation were 54.7±12.55% and 36.13±22.20% for the automated system and 53.22±13.22% and 47.26±5.74% for the conventional system, respectively. The parameters evaluated demonstrated that there was no statistical difference between the cryopreservation systems. Thus, the choice of the bovine semen cryopreservation method to be used on a farm is a responsibility of the technician, and should be based on the reality of each farm. Therefore, it is always necessary to consider that the conventional system of bovine semen cryopreservation can vary more than the automated system, which, despite the cost of the equipment, can ensure repeatability of the results and consequent quality of cryopreserved bovine semen.

O objetivo deste estudo foi comparar a eficiência do sistema automatizado (curva de resfriamento controlada eletronicamente) de congelação de sêmen bovino versus o sistema convencional (curva não controlada) por meio dos parâmetros de qualidade e viabilidade espermática no período pós-descongelação. O sêmen de quatro touros azebuados adultos foram criopreservados simultaneamente em meio tris, gema e glicerol 7%. A avaliação computadorizada do sêmen descongelado detectou os seguintes parâmetros: MP 56,50±22,25%; VAP 34,77±4,25µm/s; VSL 28,17±4,25 µm/s; VCL 58,45±6,85µm/s; STR 82,00±2,31%; LIN 49,50±3,32%, para o sistema automatizado e MP. 57,00±13,11%; VAP 25,75±1,66µm/s; VSL 23,32±1,99µm/s; VCL 63,32±1,79µm/s; STR 82,25±3,59µm/s; LIN 50,00±4,97µm/s para o sistema convencional. Os valores médios das avaliações de integridade de membrana plasmática e integridade acrossomal foram de 54,72±12,55% e 36,13±22,20% para o sistema automatizado e 53,22±13,22% e 47,26±5,74% para o sistema convencional, respectivamente. Com os parâmetros avaliados foi possível identificar que não houve diferença estatística entre os sistemas de criopreservação. Desta forma, a escolha do método de criopreservação do sêmen bovino para utilização direta na propriedade fica a critério do técnico responsável, que deverá se basear na realidade de cada propriedade. Para tanto, sempre se deve considerar que o sistema convencional pode trazer mais variações que o sistema automatizado que, apesar do custo do equipamento, pode garantir repetibilidade nos resultados e consequente qualidade do sêmen bovino criopreservado.