Resumo
Ao preservar o espermatozoide suíno no estado líquido ou criopreservado, os componentes do plasma seminal (PS) contidos nos ejaculados podem alterar a capacidade de fertilização desses gametas. O PS contém substâncias essenciais para a manutenção da viabilidade e fertilidade dos espermatozoides. No entanto, esses componentes podem ser deletérios dependendo da quantidade ou duração do tempo de contato entre a ejaculação e a remoção do PS durante o processamento do sêmen para a conservação na forma refrigerada ou congelada. Foram identificadas substâncias que prejudicam (principal proteína plasmática seminal PSPI) ou melhoram (espermadesina PSP-I) a capacidade de fertilização dos espermatozoides. Dependendo dos cachaços e dos procedimentos de colheita de sêmen, a remoção do PS pode ser benéfica antes da preservação no estado líquido ou criopreservado. Em alguns casos, o PS removido antes da congelação pode ser adicionado de volta ao diluente de descongelamento, com efeitos positivos no sêmen descongelado e na viabilidade do espermatozoide no trato reprodutivo da porca. Neste texto, há um foco nos diferentes efeitos de PS em amostras de sêmen refrigerado e criopreservado de suínos com ênfase em como PS modula a função e morfologia das células espermáticas antes, durante e após a preservação de forma refrigerada ou criopreservada.(AU)
When preserving sperm in the liquid or cryopreserved state, seminal plasma (SP) components within ejaculates can alter fertilizing capacity of these gametes. The SP contains substances essential for maintenance of sperm viability and fertility; however, these components can be deleterious depending on quantity, or duration of time before there is removal of SP from sperm in semen processing. Substances that impair (Major seminal plasma protein PSPI - boar) or improve (e.g., spermadhesin PSP-I - boar) sper- matozoa fertilizing capacity have been identified. Depending on individual males and semen collection procedures, SP removal may be beneficial before preservation in the liquid or cryopreserved state. In some cases, SP that is removed can be added back to thawing extender with there being positive effects in thawed sperm and for sperm viability in the female reproductive tract. In this review article, there is a focus on different effects of SP in samples of cooled and cryopreserved semen from boar with there being emphasis on how SP modulates the function and morphology of sperm cells before, during, and after preservation in the refrigerated or cryopreserved state.(AU)
Assuntos
Animais , Masculino , Sêmen/fisiologia , Preservação do Sêmen/veterinária , Suínos/fisiologia , Criopreservação/veterináriaResumo
O objetivo desta revisão foi compilar o que se tem na literatura a respeito do efeito da renovação de diluidor seminal, mediante centrifugação, na qualidade do sêmen refrigerado de caprinos e ovinos e no tempo de viabilidade seminal. Um dos primeiros estudos publicados com essa metodologia foi realizado com sêmen de cão, em 2005, por Verstegen et al., seguido por estudos em outras espécies, como a equina e suína. Nosso grupo de pesquisa desenvolveu alguns estudos com diferentes metodologias para avaliar a eficiência do método, a necessidade do uso da centrífuga refrigerada nesse processo, o uso de antioxidantes no diluidor para renovação e o tempo de renovação do diluidor em pequenos ruminantes.(AU)
The objective of this revision was to compile what exists in literature regarding the effect of seminal diluent renewal, through centrifugation, in the quality of cooled semen of goat and sheep and during seminal viability time. One of the first studies published with this methodology was performed with dog semen in 2005 by Verstegen et al., followed by studies in other species, such as equine and swine. Our research group developed some studies using different methodologies to evaluate method efficiency, the need to use a cooled centrifuge in this process, the use of antioxidants in the diluent for renewal and the diluent renewal time in small ruminants.(AU)
Assuntos
Ruminantes/fisiologia , Análise do Sêmen/veterinária , Tecnologia/métodos , Técnicas de Diluição do Indicador/veterináriaResumo
ABSTRACT: Spermatozoa experience oxidative, osmotic, chemical, and thermal stresses when cooled, which degrade the quality and fertilizing capacity of the cells. Adding antioxidants to the sperm extender mitigates these alterations. This study evaluated the effect of isoespintanol (ISO) on boar semen subjected to cooling. Fifteen ejaculates from five boars (Susscrofadomestica) were extended in Beltsville thawing solution (BTS) supplemented with 0 µM (control), 5 µM (ISO5), 10 µM (ISO10), 15 µM (ISO15), 20 µM (ISO20), 25 µM (ISO25), and 30 µM (ISO30) of ISO, which were then cooled for five days at 16 °C. Sperm kinetics, total motility (TM), and progressive motility (PM) were evaluated every 24 h using an IVOS computer-assisted sperm analysis (CASA) system. On day 1 and day 5 of cooling, a hypoosmotic test, spectrofluorometry, and flow cytometry were performed to evaluate the following: membrane functionality, measured as a function of hypoosmotic swelling (HOS); total antioxidant capacity (TAC); reactive oxygen species (ROS); and mitochondrial membrane potential (Δ¥M). Regression analysis and comparison of means using the Duncan test were performed. The ISO added had a slight impact on sperm motility, as evidenced by a reduction in TM at 24 h of cooling (but not prior) with the addition of 20 µM of ISO. Similarly, no effect of the ISO on the kinetics and functional integrity of the sperm membrane was observed at 96 h of cooling; however, the regression coefficients indicated that the ISO lowered the rate of decrease in sperm motility and the proportion of rapid spermatozoa relative to the concentration of ISO used. The ISO did not affect the TAC of the cooled semen; however, different concentrations of ISO lowered ROS production in the semen after 96 h of cooling. ISO also impacted the Δ¥M of the spermatozoa at 0 h of cooling, increasing the proportion of low Δ¥M cells and decreasing the proportion of high Δ¥M cells. In conclusion, ISO can reduce the loss of quality and oxidative stress occurring in boar semen during cooling and can modulate the mitochondrial activity of sperm.
RESUMO: Durante a refrigeração, os espermatozoides sofrem estresse oxidativo, osmótico, químico e térmico, que diminuem sua qualidade e afetam sua capacidade de fertilização. A adição de antioxidantes ao diluente espermático é uma alternativa para mitigar essas alterações. O objetivo desta pesquisa foi avaliar o efeito do isospintanol (ISO) na refrigeração do sêmen suíno. Quinze ejaculados de cinco varrascos (Sus scrofa domestica) foram diluídos em BTS suplementado com ISO a 0 (controle), 5 (ISO5), 10 (ISO10), 15 (ISO15), 20 (ISO20), 25 (ISO25) e 30 (ISO30) µM e foram refrigerados por cinco dias a 16 °C. A motilidade total (MT), motilidade progressiva (MP) e cinética dos espermatozóides foram avaliadas a cada 24 h com um sistema CASA IVOS. Nos dias um e cinco de refrigeração, foram avaliadas a funcionalidade da membrana, a capacidade antioxidante total (CAT), as espécies reativas de oxigênio (ROS) e o potencial de membrana mitocondrial (Δ¥M), através do teste hiposmótico (HOS), espectrofluorimetría e citometria de fluxo. Foram realizadas análises de regressão e comparação de médias, pelo teste de Duncan. A adição de ISO teve pouca influência na motilidade espermática, apresentando apenas redução na MT em 24 h de refrigeração, devido à adição de 20 µM. Da mesma forma, não foi observada influência de ISO na cinética e integridade funcional da membrana em 96 horas de refrigeração; porém, os coeficientes de regressão mostraram que ISO produziu menor taxa de diminuição da motilidade e proporção de espermatozoides rápidos dependendo da concentração utilizada. ISO não influenciou significativamente na CAT do sêmen refrigerado; entretanto, diferentes concentrações de ISO reduziram a produção de EROs a partir do sêmen após de 96 h de refrigeração. ISO também influenciou o Δ¥M dos espermatozóides em 0 h de refrigeração, com aumento das células de baixo Δ¥M e diminuição das células de alto Δ¥M. Em conclusão, o isospintanol pode reduzir a perda da qualidade e o estresse oxidativo do sêmen suíno durante a refrigeração e pode modular a atividade mitocondrial do esperma.
Resumo
Background: The use of conventional artificial insemination (AI) in sheep production is usually associated with lower fertility rates when frozen semen is used. Cooled ram semen has been an alternative over frozen semen due to the higher viability, seminal quality and fertility rates following AI. The semen preservation process promotes sperm cell modifications similar to capacitation (capacitation-like) that causes cell damage affecting viability and seminal quality, but such effects are unclear for cooled semen. The aim of this study was to determine the status of sperm cell capacitation (CA) and acrosome reaction (AR) during ram semen processing and cooling under different extenders, dilution factors, and aerobiosis conditions as a function of storage time at 5o C. Materials, Methods & Results: Two consecutive ejaculates per day per male were collected from 2 adult rams by artificial vagina at 48-72 h intervals, in three replications. After macro- and microscopic evaluations, semen was segregated into groups under 3 extenders (Tris-egg yolk or TY, citrate-egg yolk or CY, skimmed milk or SM), 2 dilution factors (1 x 109 or Bi, 100 x 106 or Mi cells/mL), and 2 aerobiosis conditions (aerobic or A, semi-anaerobic or SA). Diluted semen was cooled to 5ºC and stored for up to 72 h, with evaluations every 24 h. Aliquots of fresh ejaculates and of each cooled diluted subgroup, according to extender, dilution, and aerobiosis, were collected at times T0 and T72 for determination of acrosome status and membrane integrity by the chlortetracycline (CTC) and trypan blue-Giemsa stainings, respectively. No differences were detected in sperm cell motility (M) and motility vigor (V) between fresh and diluted semen. After cooling, a significant decrease in M was observed after 48 h in CY and SM compared with fresh semen and 0 h of cooling, while V started to decrease after 24 h in CY compared with TY. Likewise, M/V from different dilutions and aerobic conditions decreased more significantly after 48 and 24 h of cooling, respectively. The sperm capacitation status did not show differences in the proportion of non-capacitated (NCA), CA and AR sperm cells between TY, CY, and SM extenders (NCA: 75.0%, 71.3%, 74.0%; CA: 15.7%, 17.2%, 15.9%; AR: 9.3%, 11.5%, 10.2%) or between Bi and Mi dilutions (NCA: 74.0%, 72.9%; CA: 15.9%, 16.6%; AR: 10.1%, 10.5%), respectively. However, differences (P < 0.05) were observed between A and SA aerobic conditions, with CA (17.0% vs. 15.5%) and AR (11.9% vs. 8.7%) rates being higher in A than SA, respectively, with no differences in NCA (71.1% vs. 75.8%), irrespective of the storage time. Sperm cell viability decreased after 48 h, especially in CY (P < 0.05). Discussion: Ram sperm cells can suffer irreversible damage due to thermal shock during cooling. Egg yolk-based extenders provide phospholipids and cholesterol to protect the sperm cell membrane during the thermal shock caused by the change in temperature. In this study, sperm cells had irreversible decreases in M/V, with increase in acrosome and plasma membrane damage after cooling to 5ºC. The largest and smallest decreases in M and V over time were observed in the CY and TY extenders, respectively. In addition to the extender type, the semen preservation method and storage time promoted changes in the capacitation status, AR and in sperm cell viability, which per se were associated with a decrease in semen fertility. In fact, the proportions of CA and/or AR sperm cells gradually increased over time after dilution and storage at 5ºC, with a negative correlation between sperm cell viability and M/V over time. In summary, extender and cooling time affected mostly M/V, while aerobiosis condition and dilution factor were more associated with acrosome status and sperm survival, with the extender having less impact on the acrosome status as a function of time.
Assuntos
Animais , Masculino , Preservação do Sêmen/métodos , Preservação do Sêmen/veterinária , Preservação de Tecido/métodos , Ovinos , Análise do Sêmen/veterinária , Sobrevivência Celular , Técnicas de Diluição do Indicador , AerobioseResumo
Cooling and freezing processes cause physical and chemical damage to sperm by cold shock and oxidative stress. This study aimed to evaluate the effect of two antioxidants on sperm parameters of cooled and frozen-thawed ram semen diluted in an egg yolk-based extender. Semen was collected from 30 rams and processed in two consecutive experiments to test the inclusion of different concentrations of quercetin and butylated hydroxytoluene (BHT) in an egg yolk-based semen extender. Dimethyl sulfoxide (DMSO) was added as a solvent to the semen extender in a ratio of 1 mL DMSO for 90 mg of quercetin and 1 mL DMSO for 880 mg of BHT. After collection, semen was diluted at 200 × 106 motile sperm/mL (control) and split into different groups in each experiment. In experiment 1, semen was diluted with the extender containing quercetin (Q5, 5 µg/mL; Q10, 10 µg/mL; Q15, 15 µg/mL) or DMSO alone (DMSO1, 0.055 µL DMSO per mL; DMSO2, 0.165 µL DMSO per mL). In experiment 2, semen was diluted with the extender with BHT (BHT1, 0.5 µg/mL; BHT2, 1 µg/mL; BHT3, 1.5 µg/mL) or DMSO alone (DMSO3, 0.375 µL DMSO per mL; DMSO4, 1.125 µL DMSO per mL). After dilution, the semen was divided into two aliquots. Treated ram sperm samples were also subjected to different storage methods. The first set of samples was cooled at 5 °C for 24 h, whereas the second set of samples was frozen-thawed. Sperm motility parameters and plasma membrane integrity (PMI) were evaluated immediately after dilution (0h) and 24 h after cooling and in the frozen-thawed samples via computer-assisted sperm analysis and epifluorescence microscopy, respectively. The inclusion of quercetin or BHT did not affect sperm motility parameters or PMI of fresh, cooled, or frozen-thawed sperm in this study (P < 0.05). However, further studies are needed to test the effects of these antioxidants on the fertility of cryopreserved ram semen.(AU)
O resfriamento e o congelamento causam danos físicos e químicos aos espermatozoides por choque térmico e estresse oxidativo. Portanto, este estudo teve como objetivo avaliar o efeito da inclusão de dois antioxidantes em um diluente à base de gema de ovo sobre os parâmetros espermáticos do sêmen ovino resfriado e congelado. Trinta carneiros tiveram o sêmen coletado e processado em dois experimentos consecutivos para testar a inclusão de diferentes concentrações de quercetina e hidroxitolueno butilado (BHT) em diluente de sêmen à base de gema de ovo. O DMSO foi adicionado como solvente ao diluente de sêmen em uma proporção de 1 mL de DMSO parra 90 mg de quercetina e 1 Ml de DMSO para 880 mg de BHT. Após a coleta, o sêmen foi diluído a 200 × 106 espermatozoides móveis/mL (Controle) e dividido em diferentes grupos em cada experimento. Experimento 1, Quercetina (Q5, 5 µg / mL; Q10, 10 µg / mL; Q15, 15 µg / mL) ou DMSO (DMSO1, 0,055 µL de DMSO por ml; DMSO2, 0,165 µL de DMSO / mL) foram adicionados ao extensor. Experimento 2, BHT (BHT1, 0,5 µg / mL; BHT2, 1 µg / mL; BHT3, 1,5 µg / mL) ou DMSO (DMSO3, 0,375 µL de DMSO por ml; DMSO4, 1,125 µL de DMSO / mL) foram adicionados à o extensor. Após a diluição, o sêmen foi dividido em duas alíquotas. O primeiro foi resfriado a 5 ° C por 24h, enquanto o segundo foi congelado. Os parâmetros de motilidade espermática e integridade da membrana plasmática (PMI) foram avaliados, imediatamente após a diluição (0h) e 24h após o resfriamento e nas amostras congeladas, pelo CASA e microscopia de epifluorescência, respectivamente. A inclusão de quercetina ou BHT não afetou os parâmetros de motilidade espermática e PMI de espermatozoides frescos, resfriados ou congelados (P < 0,05). Portanto, a inclusão de quercetina e BHT não beneficiou os parâmetros espermáticos do sêmen ovino submetido a armazenamento líquido a 5 ° C por 24h ou protocolo de congelamento no presente estudo. No entanto, mais estudos são necessários para testar o efeito desses antioxidantes na fertilidade do sêmen ovino criopreservado.(AU)
Assuntos
Animais , Masculino , Sêmen , Hidroxitolueno Butilado , Ovinos , Análise do SêmenResumo
Equine semen has historically been chilled using milk-based media. However, the use of animal-based components presents several potential concerns, such as variability in formulations, microbial contamination and regulatory issues. We aimed to evaluate the potential of including different concentrations of soy lecithin (LS) in chemically defined Biggers, Whitten and Whittingham (BWW) medium for cooling equine semen to 15°C. Ejaculates were diluted as six different experimental groups: 1) BotuSêmen® (control); 2) BWW; 3) BWW + 1% LS; 4) BWW + 2% LS; 5) BWW + 4% LS and 6) BWW + 6% LS. BWW medium, did not preserve motility, velocity, straightness (STR), linearity (LIN), amplitude of lateral sperm head displacement (ALH), cross flagellar beat frequency (BCF), functional and structural integrity of equine spermatozoa during 24 h of refrigeration when compared to BotuSêmen® (P <0.05). The use of BWW for cooling equine semen was only possible with the addition of LS, being the concentrations equal or higher than 2% better, because they preserved total motility, curvilinear velocity (VCL) and LIN with the same potential of BotuSêmen® (P >0.05). Nevertheless, BotuSêmen® showed superiority in preserving the percentage of sperm progressive motility, average path velocity (VAP), linear progressive velocity (VSL) and BCF during cooling compared to the other extenders (P <0.05). The inclusion of soy lecithin, from 2 to 6% in the BWW medium, allowed maintaining the viability of equine semen cooled at 15ºC for up to 24 hours.
O sêmen equino tem sido historicamente refrigerado usando meios à base de leite. No entanto, o uso de componentes de origem animal causa várias preocupações potenciais, como variabilidade nas formulações, contaminação microbiana e questões regulatórias. Objetivou-se avaliar o potencial de inclusão de diferentes concentrações de lecitina de soja (LS) no meio quimicamente definido BWW - Biggers, Whitten e Whittingham para refrigeração de sêmen equino e armazenamento na temperatura de 15°C. Os ejaculados foram diluídos em seis diferentes grupos experimentais: 1) BotuSêmen® (controle); 2) BWW; 3) BWW + 1% lecitina de soja (LS); 4) BWW + 2% LS; 5) BWW + 4% LS e 6) BWW + 6% LS. O meio BWW, não preservou a motilidade, a velocidade, a retilinearidade (STR), a linearidade (LIN), a amplitude do deslocamento lateral da cabeça (ALH), a frequência de batimento flagelar cruzado (BCF), a integridade funcional e estrutural dos espermatozoides equino durante 24 h de refrigeração quando comparado ao BotuSêmen® (P <0,05). O uso de BWW para refrigeração de sêmen equino só foi possível com adição de lecitina de soja, sendo as concentrações igual ou superior a 2% melhores, pois preservaram a motilidade total, a velocidade curvilinear (VCL) e LIN com mesmo potencial do BotuSêmen® (P >0,05). Ainda assim, o diluidor comercial BotuSêmen® apresentou superioridade em preservar o percentual de espermatozoides progressivamente móveis, a velocidade média da trajetória (VAP), a velocidade linear progressiva (VSL) e a frequência do batimento flagelar cruzado (BCF) durante a refrigeração comparado aos demais diluidores (P <0,05). A inclusão de lecitina de soja, de 2 a 6% no meio BWW, permitiu a manutenção da viabilidade do sêmen equino refrigerado a 15ºC por até 24 horas.
Assuntos
Animais , Preservação do Sêmen/veterinária , Glycine max , Criopreservação/veterinária , Lecitinas , CavalosResumo
Developing effective cooled semen protocols is essential to increase pregnancy rates and reproductive efficiency in donkeys. This study aimed to evaluate the effect on sperm kinetic parameters and membrane integrity in cooled donkey semen diluted with defined milk proteins extender with 1% or 2% of egg yolk and the removal of seminal plasma. Twenty-four ejaculates from six jackasses were collected. Each ejaculate was divided into four aliquots that were diluted in extender with 1% (EY1) or 2% (EY2) egg yolk. One sample from each group was centrifuged, seminal plasma was removed (CEY1, CEY2 groups, respectively), and the samples were then refrigerated at 5 °C for 24 h. Fresh and cooled semen samples were assessed for sperm motility, morphology, and plasma membrane integrity. Total motility, progressive motility, sperm kinetic parameters, or live sperm cells were not statistically different when semen was cooled with an extender supplemented with 1% or 2% of egg yolk. Seminal plasma removal does not affect total motility or sperm kinetic parameters. However, progressive motility decreased (P<0.05) when semen was extended with 2% of egg yolk and seminal plasma was removed. Membrane integrity was affected (P<0.05) in centrifuged samples. In conclusion, the obtained results suggest that there is no difference in sperm kinetics and membrane integrity when 1% or 2% of egg yolk was added to the Equiplusï extender. Also, the removal of seminal plasma by centrifugation did not have any beneficial effect on cooled donkey semen. Further studies are needed to relate these results with in vivo fertility tests with cooled donkey semen.(AU)
O desenvolvimento de protocolos de sêmen resfriado eficazes é essencial para aumentar as taxas de prenhez e eficiência reprodutiva em jumentos. O objetivo desse estudo foi avaliar o efeito do diluente à base de proteínas do leite com 1 ou 2% de gema de ovo sobre os parâmetros cinéticos do sêmen e integridade da membrana em sêmen resfriado de jumento, com ou sem a remoção do plasma seminal. Vinte e quatro ejaculados de seis jumentos foram coletados. Cada ejaculado foi dividido em quatro alíquotas e diluído em diluente com 1% (EY1) ou 2% (EY2) de gema de ovo. Uma amostra por grupo foi centrifugada e o plasma seminal removido (grupos CEY1 e CEY2, respectivamente). Os pellets foram novamente ressuspendidos nas mesmas concentrações e diluentes. Em seguida, as quatro alíquotas foram refrigeradas a 5°C por 24 horas. Amostras de sêmen fresco e refrigerado foram avaliadas quanto à motilidade espermática e integridade da membrana plasmática. Motilidade total, motilidade progressiva, parâmetros de cinética espermática ou células espermáticas vivas não apresentaram diferença significativa quando o sêmen foi resfriado com diluente suplementado com 1% ou 2% de gema de ovo. A remoção do plasma seminal não afetou a motilidade total ou os parâmetros de cinética espermática; entretanto, a motilidade progressiva diminuiu (P<0,05) quando o sêmen foi diluído com 2% de gema de ovo e o plasma seminal removido. Nas amostras centrifugadas, a integridade da membrana foi afetada (P<0,05). Em conclusão, os resultados sugerem que não há diferença na cinética espermática e na integridade da membrana quando 1% ou 2% de gema de ovo são adicionados ao diluente Equiplusï e a remoção do plasma seminal por centrifugação não teve nenhum efeito benéfico no resfriamento de sêmen de jumento. Mais estudos são necessários para relacionar esses resultados com testes de fertilidade in vivo com sêmen resfriado em jumentos.(AU)
Assuntos
Animais , Plasma , Preservação do Sêmen/veterinária , Motilidade dos Espermatozoides , Criopreservação , Equidae , Gema de Ovo , Sêmen , ProteínasResumo
Developing effective cooled semen protocols is essential to increase pregnancy rates and reproductive efficiency in donkeys. This study aimed to evaluate the effect on sperm kinetic parameters and membrane integrity in cooled donkey semen diluted with defined milk proteins extender with 1% or 2% of egg yolk and the removal of seminal plasma. Twenty-four ejaculates from six jackasses were collected. Each ejaculate was divided into four aliquots that were diluted in extender with 1% (EY1) or 2% (EY2) egg yolk. One sample from each group was centrifuged, seminal plasma was removed (CEY1, CEY2 groups, respectively), and the samples were then refrigerated at 5 °C for 24 h. Fresh and cooled semen samples were assessed for sperm motility, morphology, and plasma membrane integrity. Total motility, progressive motility, sperm kinetic parameters, or live sperm cells were not statistically different when semen was cooled with an extender supplemented with 1% or 2% of egg yolk. Seminal plasma removal does not affect total motility or sperm kinetic parameters. However, progressive motility decreased (P<0.05) when semen was extended with 2% of egg yolk and seminal plasma was removed. Membrane integrity was affected (P<0.05) in centrifuged samples. In conclusion, the obtained results suggest that there is no difference in sperm kinetics and membrane integrity when 1% or 2% of egg yolk was added to the Equiplusï extender. Also, the removal of seminal plasma by centrifugation did not have any beneficial effect on cooled donkey semen. Further studies are needed to relate these results with in vivo fertility tests with cooled donkey semen.(AU)
O desenvolvimento de protocolos de sêmen resfriado eficazes é essencial para aumentar as taxas de prenhez e eficiência reprodutiva em jumentos. O objetivo desse estudo foi avaliar o efeito do diluente à base de proteínas do leite com 1 ou 2% de gema de ovo sobre os parâmetros cinéticos do sêmen e integridade da membrana em sêmen resfriado de jumento, com ou sem a remoção do plasma seminal. Vinte e quatro ejaculados de seis jumentos foram coletados. Cada ejaculado foi dividido em quatro alíquotas e diluído em diluente com 1% (EY1) ou 2% (EY2) de gema de ovo. Uma amostra por grupo foi centrifugada e o plasma seminal removido (grupos CEY1 e CEY2, respectivamente). Os pellets foram novamente ressuspendidos nas mesmas concentrações e diluentes. Em seguida, as quatro alíquotas foram refrigeradas a 5°C por 24 horas. Amostras de sêmen fresco e refrigerado foram avaliadas quanto à motilidade espermática e integridade da membrana plasmática. Motilidade total, motilidade progressiva, parâmetros de cinética espermática ou células espermáticas vivas não apresentaram diferença significativa quando o sêmen foi resfriado com diluente suplementado com 1% ou 2% de gema de ovo. A remoção do plasma seminal não afetou a motilidade total ou os parâmetros de cinética espermática; entretanto, a motilidade progressiva diminuiu (P<0,05) quando o sêmen foi diluído com 2% de gema de ovo e o plasma seminal removido. Nas amostras centrifugadas, a integridade da membrana foi afetada (P<0,05). Em conclusão, os resultados sugerem que não há diferença na cinética espermática e na integridade da membrana quando 1% ou 2% de gema de ovo são adicionados ao diluente Equiplusï e a remoção do plasma seminal por centrifugação não teve nenhum efeito benéfico no resfriamento de sêmen de jumento. Mais estudos são necessários para relacionar esses resultados com testes de fertilidade in vivo com sêmen resfriado em jumentos.(AU)
Assuntos
Animais , Plasma , Preservação do Sêmen/veterinária , Motilidade dos Espermatozoides , Criopreservação , Equidae , Gema de Ovo , Sêmen , ProteínasResumo
The aim of this study was to evaluate the effects of adding different concentrations of edible birds nest (EBN) which is secreted by swiftlet birds (Aerodramus fuciphagus), into EquiPlus® and E-Z Mixin® extenders on the quality of chilled Arabian stallion semen at various storage times (0, 24 and 48 h). Ten ejaculates were collected from five stallions, and diluted using the two extenders containing 0% (control), 0.12%, 0.24% and 0.24% of EBN + seminal plasma (SP). All the diluted semen samples were then cooled and stored at 5 °C, and examined at 0, 24 and 48 h. Sperm kinetic parameters were assessed using computer assisted sperm analysis (CASA) and viability were assessed using Hoechst33342/PI stain. In both extenders, total motility (TM) and progressive motility (PM) were significantly higher at 0.12% and 0.24% compared to 0.24% + SP at 24 and 48 h. At 0.12%, EZ mixin® treated semen had significantly higher TM and PM than EquiPlus® at 24 and 48 h. At 0.12% and 0.24%, average path velocity (VAP), straight-line velocity (VSL) and curvilinear velocity (VCL) were significantly higher in E-Z mixin® treated semen compared to EquiPlus® at 24 and 48 h. Comparisons between the two extender types at different concentrations of EBN showed no significant difference in lateral head amplitude (ALH), linearity (LIN), straightness (STR), beat cross frequency (BCF) and viability, irrespective of the storage time. The percentage of viable was significantly higher in E-Z mixin® than EquiPlus® at 0 and 48 h in control and 0.12%. Supplementation of the E-Z mixin® extender with 0.12% and 0.24% EBN concentrations in the absence of SP provided better CASA parameters such as TM, PM, VAP, VSL, and VCL at 24 and 48 h storage time. In conclusion, the results of this study indicated that chilled semen from Arabian stallion that was extended using E-Z mixin® and supplemented with 0.12% and 0.24% EBN concentrations performed better and yielded superior results in sperm kinetic parameters and % viable compared to EquiPlus® at 24 and 48 h storage time.(AU)
Assuntos
Animais , Masculino , Cavalos , Análise do Sêmen/veterinária , Preservação do SêmenResumo
The objective of this study was to investigate the effect of Spirulina platensis extract (SPE) addition to the freezing extender on freezability, lipid peroxidation, ultrastructure alterations and fertilizing potentials of frozen-thawed buffalo bull spermatozoa. Semen samples were collected with artificial vagina from five adult fertile bulls and diluted with Tris-base extender containing SPE (1, 5, 10 and 20 μg/mL) or without SPE (control). Diluted semen was cooled to 4 °C throughout one hour and frozen in 0.25 mL straws: prior to being stored in liquid nitrogen. Cryopresreved spermatozoa were assessed for post-thawing sperm motility, viability, acrosomal integrity, ultrastructure changes, antioxidant activities, lipid peroxidation and fertility rate. The current results clearly indicated that adding 10μg/mL SPE to the freezing extender significantly improved (P< 0.05) post-thawing motility and decrease the percentage of acrosomal damage (51.67±6.02% and 16.33±1.46%, respectively) compared with the control (28.33±4.41% and 26.33±1.77%, respectively). Moreover, addition of 10 μg/mL SPE to the semen extender significantly diminished (P< 0.05) MDA concentration (10.66±2.40 nmol/109) compared with the control (22.66±4.26 nmol/109). Therefore, the present results revealed that addition of 10μgl/mL SPE to the freezing extender might improve semen quality and reduce cryodamage of the buffalo bull spermatozoa.(AU)
Assuntos
Animais , Masculino , Búfalos , Preservação do Sêmen , Análise do Sêmen , Criopreservação/veterinária , Peroxidação de Lipídeos , FertilizaçãoResumo
Insulin is present in the seminal plasma and is involved in sperm activities like motility and capacitation. However, the effects of insulin on the viability of cooled ram sperm are not fully understood. Therefore, the objective of the current study was to evaluate the effect of insulin addition on ram sperm maintained at 5ºC. Sperm samples were collected from six healthy, mature Santa Inês rams. The ejaculates were divided into two aliquots with (insulin group) or without (control group) insulin (3 IU mL-1) in the semen extender, and then cooled at 5°C for 48 hours. Subsequently, the sperm cells were evaluated for motility and kinetics using computer-assisted semen analysis. The samples were evaluated for acrosomal integrity by fluorescein using isothiocyanate combined with peanut agglutinin (FITC-PNA) and membrane functionality by the hypoosmotic swelling test. The semen analysis was performed after 24 or 48 hours of cooling. There was an increased percentage of progressive sperm motility (%), straightness (%), linearity (%) and beat caudal frequency (Hz) in the insulin group after 24 and 48 hours of cooling (p < 0.05). However, insulin did not affect total sperm motility, sperm velocities (VSL, VAP and VCL) (µm seg-1), acrosomal integrity and membrane functionality during cooling (p > 0.05). In conclusion, the addition of 3 IU mL-1 insulin to ram semen extender improved the quality of sperm motility after cooling.(AU)
A insulina está presente no plasma seminal e participa de atividades espermáticas, como a motilidade e capacitação. Entretanto, os efeitos da insulina sobre a viabilidade do espermatozoide ovino resfriado ainda não estão elucidadas. Desta forma, o objetivo do presente estudo foi avaliar os efeitos da adição de insulina sobre o espermatozoide ovino durante o tempo de armazenamento à 5º C. Amostras espermáticas de seis carneiros da raça Santa Inês foram utilizadas. Os ejaculados foram divididos em duas aliquotas, com (grupo insulina) ou sem (grupo controle) adição de insulina (3 UI mL-1) no diluidor seminal e, posteriormente, resfriados até 5oC e mantidos armazenados por 48 horas. Em seguida, os espermatozoides foram avaliados quanto a motilidade e cinética utilizando um Sistema Computadorizado de Análise de Sêmen (CASA). Adicionalmente, as amostras espermáticas foram analizadas quanto a integridade acrosomal por meio de sondas fluorescentes (FITC-PNA) e, funcionalidade de membrana pelo teste hiposmótico. As análises seminais foram realizadas após 24 ou 48 horas de resfriamento. Foram verificados aumentos de espermatozoides com motilidade progressiva (%), retilinearidade (%), linearidade (%) e frequência de batimento caudal (BCF) (Hz) no grupo insulina após 24 ou 48 horas de resfriamento (p < 0.05). Entretanto, não houve efeito da adição de insulina sobre a porcentagem de espermatozoides moveis (%) e das velocidades espermáticas (VSL, VAP e VCL) (µm seg-1), integridade acrossomal e funcionalidade de membrana durante o resfriamento (p > 0.05). Conclui-se que adição de insulina (3 UI mL-1) no diluidor seminal melhora a qualidade da motilidade espermática durante o resfriamento.(AU)
Assuntos
Animais , Sêmen , Ovinos , Criopreservação , Análise do Sêmen , Insulina , DiluiçãoResumo
Abstract The objective of this study was to investigate the effect of Spirulina platensis extract (SPE) addition to the freezing extender on freezability, lipid peroxidation, ultrastructure alterations and fertilizing potentials of frozen-thawed buffalo bull spermatozoa. Semen samples were collected with artificial vagina from five adult fertile bulls and diluted with Tris-base extender containing SPE (1, 5, 10 and 20 μg/mL) or without SPE (control). Diluted semen was cooled to 4 °C throughout one hour and frozen in 0.25 mL straws: prior to being stored in liquid nitrogen. Cryopresreved spermatozoa were assessed for post-thawing sperm motility, viability, acrosomal integrity, ultrastructure changes, antioxidant activities, lipid peroxidation and fertility rate. The current results clearly indicated that adding 10μg/mL SPE to the freezing extender significantly improved (P< 0.05) post-thawing motility and decrease the percentage of acrosomal damage (51.67±6.02% and 16.33±1.46%, respectively) compared with the control (28.33±4.41% and 26.33±1.77%, respectively). Moreover, addition of 10 μg/mL SPE to the semen extender significantly diminished (P< 0.05) MDA concentration (10.66±2.40 nmol/109) compared with the control (22.66±4.26 nmol/109). Therefore, the present results revealed that addition of 10μgl/mL SPE to the freezing extender might improve semen quality and reduce cryodamage of the buffalo bull spermatozoa.
Resumo
The objective of this study was to compare the reproductive efficiency of dairy buffaloes undergoing fixed-time artificial insemination (FTAI) protocols based on progesterone/estrogen (P4/E2) and eCG during unfavorable breeding season using cooled (CS) and frozen semen (FS). A total of 446 buffaloes (> 40 days postpartum) were randomly distributed into four blocks (years): B1-2014 (n = 143), B2-2015 (n = 34), B3-2016 (n = 90), and B4-2017 (n = 179). Each block was subdivided into two (AI with CS and FS using the same ejaculate of each bull). Thus, the block subdivision was as follows: B1 (CS = 71 and FS = 72); B2 (CS = 18 and FS = 16); B3 (CS = 47 and FS = 43); and B4 (CS = 90 and FS = 89). The ejaculates of eight Murrah bulls collected using an artificial vagina were divided into two aliquots: one aliquot was diluted in Botu-Bov® commercial extender and cooled (BB-CS), and the other was diluted in the same extender and frozen (BB-FS). BB-CS aliquots were cooled at 5 °C/24 h using a refrigerator. BB-FS group aliquots were also cooled, and after equilibrating at 5 °C for 4 h, were placed in a 21-L Styrofoam box, 5 cm above the surface of liquid nitrogen. In the afternoon (A) on D0 (2:00 p.m.) the animals received EB 2.0 mg IM (Estrogin®) and an ear implant (CRESTAR® 3.0 mg P4). At D9 (A), the implant was removed, and the animals received eCG 400 IU IM (Folligon® 5000) + Cloprostenol PGF2α 0.530 mg IM (Sincrocio®). At D10 (A), the animals received EB 1.0 mg IM (Estrogin®), and at D12 (8:00 a.m.), AI was performed. At D42, pregnancy was diagnosed via ultrasonography. Total CRs were 48.2% CS and 34.6% FS for years 2014 to 2017, with a significant difference of 13.7% (P<0.05). In conclusion, cooled semen resulted in higher CR than frozen semen in dairy buffaloes under the P4/E2 and eCG FTAI during the unfavorable reproductive season.(AU)
O objetivo deste estudo foi comparar a eficiência reprodutiva de búfalas leiteiras submetidas a protocolos de inseminação artificial em tempo fixo (IATF) à base de progesterona/estrogênio (P4/E2) e eCG, durante a estação reprodutiva desfavorável, usando-se sêmen resfriado (SR) e congelado (SC) Um total de 446 búfalas (> 40 dias após o parto) foi distribuído aleatoriamente em quatro blocos (anos): B1-2014 (n = 143), B2-2015 (n = 34), B3-2016 (n = 90) e B4-2017 (n = 179). Cada bloco foi subdividido em dois (IA com SR e SC utilizando-se a mesma ejaculação de cada touro). Assim, a subdivisão do bloco foi a seguinte: B1 (SR = 71 e SC = 72); B2 (SR = 18 e SC = 16); B3 (SR = 47 e SC = 43); e B4 (SR = 90 e SC = 89). Os ejaculados de oito touros Murrah coletados com vagina artificial foram divididos em duas alíquotas: uma alíquota diluída em diluente comercial Botu-Bov® e resfriada (BB-SR), e a outra diluída no mesmo diluente e congelada (BB-SC). As alíquotas de BB-SR foram resfriados a 5°C/24h usando-se um refrigerador. As alíquotas do grupo BB-SC também foram resfriadas e, após equilíbrio a 5°C por 4h, foram colocadas em uma caixa de isopor de 21L, 5 cm acima da superfície do nitrogênio líquido. À tarde (A), no D0 (14h), os animais receberam BE 2,0 mg IM (Estrogin®) e um implante auricular (Crestar® 3,0 mg P4). No D9 (A), o implante foi retirado e os animais receberam eCG 400 UI IM (Folligon® 5000) + cloprostenol PGF2α 0,530 mg IM (Sincrocio®). No D10 (A), os animais receberam BE 1,0mg IM (Estrogin®), e, no D12 (8h da manhã), foram realizadas as IAs. No D42, a gestação foi diagnosticada por ultrassonografia. As taxas de concepção (TC) totais foram 48,2% SR e 34,6% SC para os anos de 2014 a 2017, com uma diferença significativa de 13,7% (P<0,05). Em conclusão, o sêmen resfriado resultou em maior TC do que o sêmen congelado em bubalinos leiteiros sob P4/E2 e eCG FTAI durante a estação reprodutiva desfavorável.(AU)
Assuntos
Animais , Feminino , Preservação do Sêmen/veterinária , Búfalos/fisiologia , Sincronização do Estro , Progesterona/administração & dosagem , Inseminação Artificial/veterinária , Estrogênios/administração & dosagemResumo
Abstract The aim of this study was to evaluate the effects of adding different concentrations of edible bird's nest (EBN) which is secreted by swiftlet birds (Aerodramus fuciphagus), into EquiPlus® and E-Z Mixin® extenders on the quality of chilled Arabian stallion semen at various storage times (0, 24 and 48 h). Ten ejaculates were collected from five stallions, and diluted using the two extenders containing 0% (control), 0.12%, 0.24% and 0.24% of EBN + seminal plasma (SP). All the diluted semen samples were then cooled and stored at 5 °C, and examined at 0, 24 and 48 h. Sperm kinetic parameters were assessed using computer assisted sperm analysis (CASA) and viability were assessed using Hoechst33342/PI stain. In both extenders, total motility (TM) and progressive motility (PM) were significantly higher at 0.12% and 0.24% compared to 0.24% + SP at 24 and 48 h. At 0.12%, E-Z mixin® treated semen had significantly higher TM and PM than EquiPlus® at 24 and 48 h. At 0.12% and 0.24%, average path velocity (VAP), straight-line velocity (VSL) and curvilinear velocity (VCL) were significantly higher in E-Z mixin® treated semen compared to EquiPlus® at 24 and 48 h. Comparisons between the two extender types at different concentrations of EBN showed no significant difference in lateral head amplitude (ALH), linearity (LIN), straightness (STR), beat cross frequency (BCF) and viability, irrespective of the storage time. The percentage of viable was significantly higher in E-Z mixin® than EquiPlus® at 0 and 48 h in control and 0.12%. Supplementation of the E-Z mixin® extender with 0.12% and 0.24% EBN concentrations in the absence of SP provided better CASA parameters such as TM, PM, VAP, VSL, and VCL at 24 and 48 h storage time. In conclusion, the results of this study indicated that chilled semen from Arabian stallion that was extended using E-Z mixin® and supplemented with 0.12% and 0.24% EBN concentrations performed better and yielded superior results in sperm kinetic parameters and % viable compared to EquiPlus® at 24 and 48 h storage time.
Resumo
Objetivou-se avaliar o efeito da adição de diferentes concentrações do colesterol carregado por ciclodextrina (CCC) sobre os espermatozoides congelados de ovinos. Foram coletados dois ejaculados de 10 carneiros (n=20) e diluídos em Tris-Gema de ovo até a concentração final de 200 x106 sptz/mL e mantidos em banho maria a 32 °C. O CCC foi adicionado: controle (0,0mg), 1,5mg, 3,0mg e 6,0mg de CCC/120 x106 sptz/mL. Após adição, o sêmen foi resfriado a 5 °C por duas horas, após esse período, envasado em palhetas de 0,5mL e então acondicionado sob vapor de nitrogênio líquido (N2L), a 8 cm da lâmina líquida/15 minutos e depois imersos no N2L. As amostras foram analisadas quanto à motilidade espermática, integridade da membrana plasmática e da membrana acrossomal, atividade mitocondrial e teste de ligação. As variáveis foram submetidas à análise de variância e médias comparadas pelo teste de Tukey a 5% de probabilidade. O maior percentual de integridade da membrana plasmática, acrossomal e a maior atividade mitocondrial foram obtidos utilizando 6,0mg de CCC. A adição de3,0mg de CCC manteve o percentual de motilidade espermática após a criopreservação, quando comparado aos demais tratamentos e controle. A adição de 1,5 e 3,0mg de CCC mantiveram o percentual de viabilidade espermática após a criopreservação acima de 65%. O número de espermatozoides com capacidade de ligação a membrana perivitelina da gema de ovo foi maior (p<0,05) no tratamento com 3,0mg de CCC. Concluiu se que a adição de CCC ao sêmen diluído, nas concentrações avaliadas, melhora a qualidade espermática após descongelação.
The objective was to evaluate the effect of adding different concentrations of cholesterol carried by cyclodextrin (CCC) on frozen ovine sperm. Two ejaculates were collected from 10 rams (n=20) and diluted in Tris-Yolk until the final concentration of 200 x 106 sptz/mL was reached and kept in a water bath at 32 °C. The CCC was added: control (0,0mg), 1.5mg, 3.0mg, and 6.0mg of CCC/120 x 106 sptz/mL. After the addition, the semen was cooled at 5 °C for two hours, after that period, filled in 0.5 mL straws, and then conditioned under liquid nitrogen vapor (N2L), at 8 cm of the liquid/15 minutes, and then immersed in N2L. The samples were analyzed for sperm motility, plasma membrane and acrosomal membrane integrity, mitochondrial activity, and binding test. The variables were subjected to analysis of variance and means compared by Tukey's test at 5% probability. The highest percentage of plasma membrane integrity and the highest mitochondrial activity were obtained using 6.0mg of CCC. The addition of 3.0mg of CCC maintained the percentage of sperm motility after cryopreservation, when compared to other treatments and control. The addition of 1.5 and 3.0mg of CCC maintained the percentage of sperm viability after cryopreservation, above 65%. The count of sperm with ability to bind to the egg yolk perivitelline membrane was higher (p<0.05) with 3.0mg of CCC. It is concluded that the addition of CCC to the diluted semen, in the evaluated concentrations, improves the sperm quality after thawing.
Assuntos
Masculino , Animais , Criopreservação/métodos , Criopreservação/veterinária , Espermatozoides/efeitos dos fármacos , Oligossacarídeos/farmacologia , Ovinos , Sêmen/efeitos dos fármacosResumo
Objetivou-se avaliar o efeito da adição de diferentes concentrações do colesterol carregado por ciclodextrina (CCC) sobre os espermatozoides congelados de ovinos. Foram coletados dois ejaculados de 10 carneiros (n=20) e diluídos em Tris-Gema de ovo até a concentração final de 200 x106 sptz/mL e mantidos em banho maria a 32 °C. O CCC foi adicionado: controle (0,0mg), 1,5mg, 3,0mg e 6,0mg de CCC/120 x106 sptz/mL. Após adição, o sêmen foi resfriado a 5 °C por duas horas, após esse período, envasado em palhetas de 0,5mL e então acondicionado sob vapor de nitrogênio líquido (N2L), a 8 cm da lâmina líquida/15 minutos e depois imersos no N2L. As amostras foram analisadas quanto à motilidade espermática, integridade da membrana plasmática e da membrana acrossomal, atividade mitocondrial e teste de ligação. As variáveis foram submetidas à análise de variância e médias comparadas pelo teste de Tukey a 5% de probabilidade. O maior percentual de integridade da membrana plasmática, acrossomal e a maior atividade mitocondrial foram obtidos utilizando 6,0mg de CCC. A adição de3,0mg de CCC manteve o percentual de motilidade espermática após a criopreservação, quando comparado aos demais tratamentos e controle. A adição de 1,5 e 3,0mg de CCC mantiveram o percentual de viabilidade espermática após a criopreservação acima de 65%. O número de espermatozoides com capacidade de ligação a membrana perivitelina da gema de ovo foi maior (p<0,05) no tratamento com 3,0mg de CCC. Concluiu se que a adição de CCC ao sêmen diluído, nas concentrações avaliadas, melhora a qualidade espermática após descongelação.(AU)
The objective was to evaluate the effect of adding different concentrations of cholesterol carried by cyclodextrin (CCC) on frozen ovine sperm. Two ejaculates were collected from 10 rams (n=20) and diluted in Tris-Yolk until the final concentration of 200 x 106 sptz/mL was reached and kept in a water bath at 32 °C. The CCC was added: control (0,0mg), 1.5mg, 3.0mg, and 6.0mg of CCC/120 x 106 sptz/mL. After the addition, the semen was cooled at 5 °C for two hours, after that period, filled in 0.5 mL straws, and then conditioned under liquid nitrogen vapor (N2L), at 8 cm of the liquid/15 minutes, and then immersed in N2L. The samples were analyzed for sperm motility, plasma membrane and acrosomal membrane integrity, mitochondrial activity, and binding test. The variables were subjected to analysis of variance and means compared by Tukey's test at 5% probability. The highest percentage of plasma membrane integrity and the highest mitochondrial activity were obtained using 6.0mg of CCC. The addition of 3.0mg of CCC maintained the percentage of sperm motility after cryopreservation, when compared to other treatments and control. The addition of 1.5 and 3.0mg of CCC maintained the percentage of sperm viability after cryopreservation, above 65%. The count of sperm with ability to bind to the egg yolk perivitelline membrane was higher (p<0.05) with 3.0mg of CCC. It is concluded that the addition of CCC to the diluted semen, in the evaluated concentrations, improves the sperm quality after thawing.(AU)
Assuntos
Animais , Masculino , Ovinos , Criopreservação/métodos , Criopreservação/veterinária , Sêmen/efeitos dos fármacos , Oligossacarídeos/farmacologia , Espermatozoides/efeitos dos fármacosResumo
Dois experimentos foram realizados para verificar a viabilidade de diluentes para sêmen equino refrigerado. O objetivo do primeiro experimento foi verificar a eficiência do leite UHT integral e semidesnatado, comparado ao leite desnatado. Amostras foram analisadas a fresco e posteriormente diluídas em leite UHT integral, semidesnatado e desnatado. Foram realizados exames de motilidade espermática e vigor, CFDA/PI e HOST pós-diluição (0h), e no sêmen refrigerado a 5 ºC após 24 e 48 horas. Não houve diferença entre os três diluentes, quanto à motilidade espermática (p=0,9880), vigor (p=0,7249), CFDA/PI (p=0,3382) e HOST (p > 0,01). Houve uma diminuição na qualidade do sêmen, no decorrer do tempo (p < 0,01), independente do diluente utilizado. Pode-se afirmar que, na falta de leite UHT desnatado, o semidesnatado e o integral podem ser usados, uma vez que eles não provocam prejuízo na qualidade do sêmen refrigerado armazenado por até 48 horas. No segundo experimento, o objetivo foi verificar a eficácia do leite desnatado em comparação com diluentes comerciais (Botusemen® (BS) e Botusemen Special® (BSS)). Logo após a coleta do sêmen, as amostras foram diluídas com leite UHT desnatado (LD), Botusemen® (BS) e Botusemen Special®(BSS). A análise de sêmen seguiu o mesmo protocolo do primeiro experimento. As amostras de sêmen refrigeradas com BSS apresentaram HOST e CFDA/PI (p< 0,001) maiores nas 24h e 48 h o que indica que o diluente BSS promove aumento da longevidade dos espermatozoides em comparação com os outros analisados.
Two trials were performed to verify the viability of extenders equine cooled semen. The objective of the first trial was to verify the efficacy of whole and semi-skimmed UHT milk compared to skim milk. Fresh semen samples were analyzed and later diluted in UHT whole milk, semi skimmed and skimmed milk. Sperm motility and vigor, CFDA / PI and HOST tests were performed post-dilution (0h), and in semen cooled at 5oC after 24 and 48h. There was no difference between the 3 extenders, for sperm motility (p = 0.9880), vigor (p = 0.7249), CFDA / PI (p = 0.3882) and HOST (p> 0.01). There was a decrease in semen quality over time (p <0.01), regardless of the extender used. It can be stated that in the absence of skimmed UHT milk, semi-skimmed and whole milk can be used since they do not impair the quality of refrigerated semen stored for up to 48 hours. In the second trial the objective was to verify the efficacy of the skim milk compared to commercial extenders (Botusemen® (BS) and Botusemen Special® (BSS)). Soon after semen collection, the samples were diluted with UHT skim milk (LD), Botusemen® (BS) and Botusemen Special® (BSS). Semen analysis followed the same protocol as the first experiment. BSS-cooled semen showed higher HOST and CFDA / PI (p <0.001) in 24h and 48h indicating that BSS diluent promotes increased sperm longevity compared to the others analyzed.
Assuntos
Masculino , Animais , Cavalos , Diluição , Leite/química , Preservação do Sêmen/métodos , Preservação do Sêmen/veterináriaResumo
Dois experimentos foram realizados para verificar a viabilidade de diluentes para sêmen equino refrigerado. O objetivo do primeiro experimento foi verificar a eficiência do leite UHT integral e semidesnatado, comparado ao leite desnatado. Amostras foram analisadas a fresco e posteriormente diluídas em leite UHT integral, semidesnatado e desnatado. Foram realizados exames de motilidade espermática e vigor, CFDA/PI e HOST pós-diluição (0h), e no sêmen refrigerado a 5 ºC após 24 e 48 horas. Não houve diferença entre os três diluentes, quanto à motilidade espermática (p=0,9880), vigor (p=0,7249), CFDA/PI (p=0,3382) e HOST (p > 0,01). Houve uma diminuição na qualidade do sêmen, no decorrer do tempo (p < 0,01), independente do diluente utilizado. Pode-se afirmar que, na falta de leite UHT desnatado, o semidesnatado e o integral podem ser usados, uma vez que eles não provocam prejuízo na qualidade do sêmen refrigerado armazenado por até 48 horas. No segundo experimento, o objetivo foi verificar a eficácia do leite desnatado em comparação com diluentes comerciais (Botusemen® (BS) e Botusemen Special® (BSS)). Logo após a coleta do sêmen, as amostras foram diluídas com leite UHT desnatado (LD), Botusemen® (BS) e Botusemen Special®(BSS). A análise de sêmen seguiu o mesmo protocolo do primeiro experimento. As amostras de sêmen refrigeradas com BSS apresentaram HOST e CFDA/PI (p< 0,001) maiores nas 24h e 48 h o que indica que o diluente BSS promove aumento da longevidade dos espermatozoides em comparação com os outros analisados.(AU)
Two trials were performed to verify the viability of extenders equine cooled semen. The objective of the first trial was to verify the efficacy of whole and semi-skimmed UHT milk compared to skim milk. Fresh semen samples were analyzed and later diluted in UHT whole milk, semi skimmed and skimmed milk. Sperm motility and vigor, CFDA / PI and HOST tests were performed post-dilution (0h), and in semen cooled at 5oC after 24 and 48h. There was no difference between the 3 extenders, for sperm motility (p = 0.9880), vigor (p = 0.7249), CFDA / PI (p = 0.3882) and HOST (p> 0.01). There was a decrease in semen quality over time (p <0.01), regardless of the extender used. It can be stated that in the absence of skimmed UHT milk, semi-skimmed and whole milk can be used since they do not impair the quality of refrigerated semen stored for up to 48 hours. In the second trial the objective was to verify the efficacy of the skim milk compared to commercial extenders (Botusemen® (BS) and Botusemen Special® (BSS)). Soon after semen collection, the samples were diluted with UHT skim milk (LD), Botusemen® (BS) and Botusemen Special® (BSS). Semen analysis followed the same protocol as the first experiment. BSS-cooled semen showed higher HOST and CFDA / PI (p <0.001) in 24h and 48h indicating that BSS diluent promotes increased sperm longevity compared to the others analyzed.(AU)
Assuntos
Animais , Masculino , Leite/química , Preservação do Sêmen/métodos , Preservação do Sêmen/veterinária , Cavalos , DiluiçãoResumo
This study aimed to evaluate if the addition of chlorogenic acid (ChA) to semen extenders improves the quality of cooled boar semen processed in Percoll. The experimental design was randomized blocks (ejaculates) in a 2×3 factorial (with or without Percoll, and three antioxidant systems: a negative control, without supplementation, a positive control vitamin E, and ChA), totaling six treatments and 12 repetitions. ChA and vitamin E (VE) were added at 4.5 mg/ml and 400 μg/ml in extender, respectively. At 0, 48 and 72h of storage at 15ºC, 80 ml insemination doses each containing 2.0 billion sperm cells were submitted to centrifugation in Percoll. The use of Percoll impaired (P<0.01) all motility patterns but decreased (P<0.01) the number of abnormal cells at 0, 48 and 72h of storage. Both VE and ChA improved (P<0.05) the total motility after Percoll processing, but only in semen stored for 48h. The same effect was not observed (P>0.05) in semen stored for 72h. ChA improved (P<0.05) the total motility of the semen stored for 72h, but this effect was not observed (P>0.05) when the semen was processed in Percoll. The antioxidants had no effect (P>0.05) on the viability and integrity of the acrosome, but ChA reduced (P<0.05) the number of abnormal cells at 0h, while VE increased the number of abnormal cells in semen stored for 72h, independent of the use of Percoll. There was no effect (P>0.05) of antioxidants or Percoll on the concentration of malondialdehyde in seminal plasma. The use of Percoll had no effect (P>0.05) on the cholesterol efflux, but ChA increased (P<0.05) this parameter at 0h and reduced (P<0.05) in the semen stored for 72h not processed with Percoll. In conclusion, the addition of ChA to semen extenders improved the quality of boar semen processed or not in Percoll.(AU)
Assuntos
Animais , Suínos/fisiologia , Ácido Clorogênico/administração & dosagem , Ácido Clorogênico/efeitos adversos , Análise do Sêmen/métodos , Análise do Sêmen/veterináriaResumo
This study aimed to compare the effects a commercial milk-based extender and a self-made egg yolk extender had on the quality of canine semen stored at two different temperatures, 5ºC or 15ºC. The ejaculate obtained was split into two aliquots of equal volume and diluted with the milk or egg yolk extender. The final concentration was 100×106 spermatozoa/mL. Diluted semen was placed in transport containers and maintained at final storage temperatures of 5ºC and 15ºC. The quality of the chilled semen was assessed 12, 24, and 36 hours after storage. Semen diluted with the milk extender had higher motility, vigour, and plasma membrane integrity (p<0.05) of the spermatozoa than that diluted with the egg yolk extender. No difference in the semen quality was observed between the stored temperatures in both the groups. The difference observed between the extenders could be due to the standard formulation of the commercial milk extender and the presence of glucose in the mixture. In conclusion, the milk extender was better than the egg yolk extender at preserving the motility, viability, and membrane integrity of chilled canine semen for up to 36 hours. The storage temperature did not seem to affect the semen quality, suggesting that canine semen can be refrigerated at 15ºC.
O objetivo desse estudo foi avaliar a influência de um diluente comercial à base de leite, comparado à um diluente preparado com de gema de ovo na qualidade do sêmen de cão, armazenado em duas diferentes temperaturas (5º C ou 15º C). O ejaculado obtido foi dividido em duas alíquotas de volumes iguais, que foram diluídas com o diluente leite ou o diluente gema de ovo, apresentando uma concentração final de 100x106 espermatozoides/mL. O sêmen diluído foi colocado em caixas de transporte, mantendo temperaturas finais de refrigeração de 5º C e 15º C. A qualidade do sêmen refrigerado foi avaliada após 12, 24 e 36h de armazenamento. O sêmen diluído com o diluente leite resultou em maior motilidade, vigor e integridade de membrana plasmática (p<0,05) dos espermatozoides que o diluído com o diluente gema de ovo. Dentro de cada grupo, não foi encontrada nenhuma influencia da temperatura de armazenamento em relação à qualidade do sêmen. A diferença observada entre os diluentes, pode ter ocorrido devido à formulação padrão do diluente comercial à base de leite, além da presença de glicose em sua composição. Em conclusão, o diluente leite apresentou superior preservação da motilidade, viabilidade e integridade de membrana plasmática do sêmen de cão refrigerado, por até 36h de armazenamento, que o diluente gema de ovo, e a temperatura de armazenamento não interferiu na qualidade seminal, sugerindo que 15º C também pode ser utilizado para a refrigeração do sêmen canino.