RESUMEN
In vitro embryo production (IVEP) is an extremely important tool for genetic improvement in livestock and it is the biotechnology that has grown the most recently. However, multiple ovulation followed by embryo transfer is still considered the leading biotechnology for embryo production in small ruminants. This review aimed to identify what is still missing for more efficient diffusion of IVEP in small ruminants, going through the IVEP steps and highlighting the main factors affecting the outcomes. Oocyte quality is essential for the success of IVEP and an aspect to be considered in small ruminants is their reproductive seasonality and strategies to mitigate the effect of season. The logistics for oocyte collection from live females is more complex than in cattle, and tools to simplify this collection system and/or to promote an alternative way of recovering oocytes may be an important point in this scenario. The heterogeneity of oocytes collected from growing follicles in live females or from ovaries collected from abattoirs remains a challenge, and there is a demand to standardize/homogenize the hormonal stimulatory protocols and IVM protocols for each source of oocytes. The use of sexed semen is technically possible, however the low market demand associated with the high costs of the sexing process prevents the routine use of this technique, but its higher availability is an important aspect aiming for greater dissemination of IVEP. New noninvasive approaches for embryo selection are key factors since the selection for transfer or cryopreservation is another difficulty faced among laboratories. Embryo selection is based on morphological traits, although these are not necessarily reliable in predicting pregnancy. Several issues described in this review must be considered by researchers in other to promote the diffusion of IVEP in small ruminants.
RESUMEN
BACKGROUND: Information on the impact of hormonal protocols for cervical dilation on the quality of ovine embryos is scarce. METHODS: To compare the quality of embryos after cervical dilation protocol, ewes (n = 64) were allocated into either a treated group (100 µg estradiol benzoate intravenous and 0.12 mg cloprostenol intramuscularly, 12 hours before embryo collection plus 100 iu oxytocin intravenous 15 minutes before the collection procedure) or a control group (saline). Luteal function was analysed using ultrasonography and P4 measurement. Some collected embryos were frozen/thawed for gene expression, others were cultured in vitro, frozen/thawed for gene expression, and the remaining embryos were fixed for the apoptosis test (TUNEL test). RESULTS: The treatment reduced fluid (p=0.04) and structure (p=0.03) recovery rates, but the morphological quality, development stage, and apoptosis incidence of the embryos were not affected by treatment. The corpora lutea of the control group had greater blood perfusion (p = 0.002) and greater P4 concentrations at 6, 9, and 12 h after the treatment (p < 0.0001). The expression of BAX, BCL2, PRDX1, and HSP90 genes were not affected by the treatment. However, the embryos in the treated group had fewer NANOG and OCT4 transcripts than control embryos (p = 0.008; p = 0.006, respectively). After culture, there was no difference between the groups in any gene. CONCLUSION: The hormonal protocol for cervical dilation reduced the efficiency of embryo collection. In addition, the treatment induced luteolysis and a transient alteration of embryo gene expression, however there were no detectable changes in embryo morphological quality, development stage, or incidence of apoptosis.
Asunto(s)
Transferencia de Embrión , Embrión de Mamíferos , Animales , Cloprostenol/farmacología , Dilatación/veterinaria , Transferencia de Embrión/métodos , Transferencia de Embrión/veterinaria , Femenino , Expresión Génica , Progesterona , OvinosRESUMEN
Resveratrol, a potent antioxidant, can be an alternative semen extender constituent to protect spermatozoa against reactive oxygen species (ROS); however, effects on sperm quality post-thawing and sperm function is not well understood. This study, therefore, was conducted to investigate effects of resveratrol supplementation to semen extender on sperm quality post-thawing. Bull semen was cryopreserved using extenders not supplemented or supplemented with 0.05, 0.1, or 1 mM resveratrol. Supplementation of extender with resveratrol at 0.05 mM resulted in greater (P < 0.05) sperm progressive motility, average path velocity, straight linear velocity, linearity and straightness when compared with no or 1 mM supplementations. Furthermore, effects of 0.05 mM resveratrol supplementations on plasma membrane and acrosome integrity and sperm fertilization capacity using in vitro procedures were investigated. Supplementation of semen extender with resveratrol resulted in a greater (P < 0.05) proportion of frozen-thawed spermatozoa with an intact acrosome and plasma membrane. Results from in vitro fertilization studies indicated there were no differences (P> 0.05) when there was no supplementation or supplementation with 0.05 mM resveratrol on embryo development to the cleavage and blastocyst stages. In conclusion, addition of resveratrol to bull semen extender resulted in greater sperm quality post-thawing in a dose-dependent manner, with values for variables related to sperm quality being greater when there was resveratrol supplementation at the 0.05 mM concentration. Proportion of embryo developing to the cleavage and blastocyst stages after in vitro fertilization was not affected by resveratrol supplementation to semen extenders.
Asunto(s)
Bovinos , Criopreservación/veterinaria , Resveratrol/farmacología , Análisis de Semen/veterinaria , Preservación de Semen/veterinaria , Animales , Antioxidantes/administración & dosificación , Antioxidantes/farmacología , Relación Dosis-Respuesta a Droga , Fertilización In Vitro/veterinaria , Masculino , Resveratrol/administración & dosificaciónRESUMEN
This study was conducted to assess effects of different doses of pFSH on follicular recruitment, superovulatory response, ova/embryo recovery, and embryo yield in lactating ewes. Ewes (nâ¯=â¯24) had a superovulation treatment regimen imposed. All ewes were implanted with a progesterone intravaginal device for 9 d, and administered either 100 (G-100) or 200 (G-200) mg pFSH, proportioned into six doses administered at 12-h intervals, starting 60â¯h before device removal. At 7 days subsequent to progesterone device removal, there were non-surgical embryo recoveries (NSER) from ewes having three or more corpora lutea. At the time of the first pFSH injection, number of antral follicles were similar (Pâ¯<â¯0.05) between ewes in the G-100 and G-200 group, however, there were more 3.1-4.0â¯mm follicles in ewes of the G-200 than G-100 group at the time of the second pFSH administration. Estrous response and CL number were less (Pâ¯<â¯0.05) in ewes of the G-100 (66.7 % and 2.6⯱â¯0.7) than G-200 (91.7 % and 11.6⯱â¯1.2) group. There were embryo collections from 100 % and 90.9 % of ewes in the G-100 and G-200 groups, respectively (Pâ¯>â¯0.05). Viable embryo numbers and ova/embryo recovery rate were greater (Pâ¯<â¯0.05) in ewes of the G-200 (6.9⯱â¯1.1 and 67.8 %) than G-100 (1.0⯱â¯0.5 and 27.6 %) group. A dose of 200 mg pFSH was more effective in inducing a superovulatory response and embryo yield after NSER in ewes, however, the 100 mg dose was insufficient for these purposes.
Asunto(s)
Hormona Folículo Estimulante/farmacología , Ovinos/embriología , Superovulación/efectos de los fármacos , Animales , Cuerpo Lúteo/efectos de los fármacos , Estudios Cruzados , Relación Dosis-Respuesta a Droga , Ciclo Estral/efectos de los fármacos , Femenino , Hormona Folículo Estimulante/administración & dosificación , EmbarazoRESUMEN
Conjugated linoleic acid (CLA) is a mixture of positional isomers of linoleic acid found in meat and dairy products from ruminants. It is a trans fat widely used by athletes as a food supplement, due to a supposed effect of maximizing the use of body fat reserves. The interest in diet and culture media supplementation with CLA is an emerging area, demanding studies in order to elucidate its benefits in the reproductive parameters, as well as in cryopreservation. Therefore, the aim of this review was to discuss the effects of CLA on the oocytes, sperm and embryos cryotolerance. Some studies have already demonstrated its use in cryopreservation of germline. Among those, it was observed that CLA supplementation during oocyte in vitro maturation can increase their viability post-freezing and developmental capacity. Regarding the use of CLA on sperm, there are few studies and their results are still inconclusive. Finally, studies about CLA supplementation on embryo culture media have shown promising results, indicating that this bioactive molecule is able to modulate lipid uptake on blastomeres. Altogether, these findings demonstrate the potential use of CLA as a bioactive molecule to improve germline and embryo cryotolerance and open new perspectives on human and animal reproduction field.(AU)
O ácido linoleico conjugado (CLA) é uma mistura de isômeros posicionais do ácido linoleico encontrado em carne e laticínios de ruminantes. É um tipo de gordura trans muito utilizada por atletas para como suplemento alimentar devido a um suposto efeito de maximizar a utilização das reservas de gordura corporal. O interesse na suplementação de dietas e meios de cultura com o CLA é uma área emergente, exigindo estudos para elucidar seus benefícios nos parâmetros reprodutivos e na criopreservação. Dessa forma, o objetivo dessa revisão foi discutir os efeitos do CLA na criotolerância de oócitos, espermatozóides e embriões. Alguns estudos já demonstraram seu uso na criopreservação da linhagem germinativa. Entre esses, foi observado que a suplementação de CLA durante a maturação in vitro de oócitos pode aumentar sua viabilidade pós-congelamento e capacidade de desenvolvimento. Em relação ao uso de CLA no esperma, existem poucos estudos e seus resultados ainda são inconclusivos. Por último, estudos sobre a suplementação de CLA em meios de cultura de embriões mostraram resultados promissores, indicando que essa molécula bioativa é capaz de modular a captação de lipídios em blastômeros. No total, essas descobertas demonstram o potencial uso do CLA como uma molécula bioativa para melhorar a linha germinativa e a criotolerância ao embrião e abrir novas perspectivas no campo da reprodução humana e animal.(AU)
Asunto(s)
Animales , Ácidos Linoleicos Conjugados/uso terapéutico , Oocitos , Espermatozoides , Embrión de Mamíferos , Respuesta al Choque por Frío/fisiología , Criopreservación/veterinaria , Suplementos DietéticosRESUMEN
This study assessed the effect of progestogen treatment length on ovarian parameters and embryo yield in superovulated Lacaune ewes collected by nonsurgical embryo recovery. Twenty-three lactating ewes were superovulated 30 d apart using a cross-over design. All ewes received 60 mg of MAP intravaginal sponges for 6 (G-6 group) or 9 (G-9 group) d. A total dose of 133 mg pFSH was given in six decreasing doses (twice a day) starting at 60 h before device removal. Ultrasound examination of the ovaries was performed at the first pFSH injection and one day before embryo recovery, which was performed 6-7 d after the onset of estrus. Embryo recovery was conducted only in ewes that expressed estrus and were mated. There was no difference (P > 0.05) in the total number of follicles between G-6 (15.7 ± 1.0) and G-9 (15.6 ± 0.8) at the time of the first pFSH treatment. The percentage of responding donors with ≥3 corpora lutea (CL; 78.2% [18/23] vs 69.5% [16/23]), mean (±SEM) CL number (7.0 ± 1.2 vs 8.1 ± 1.6), transcervical passage rate (94.4% [17/18] vs 83.3% [15/18], and ova/embryo recovery rate (54.5% [60/110] vs 68.0% [83/122]) were not different (P > 0.05) between the G-6 and G-9 groups. However, the mean number of viable embryos was lower (P < 0.05) in the G-6 group (1.8 ± 0.7) than in the G-9 group. (3.5 ± 1.1). In conclusion, treatment with an intravaginal MAP sponge for 9 d during a superovulation protocol is beneficial for viable embryo yield in Lacaune ewes out of the breeding season.
Asunto(s)
Progestinas , Superovulación , Animales , Cuerpo Lúteo , Femenino , Hormona Folículo Estimulante , Lactancia , OvinosRESUMEN
This study assessed the efficiency of cervical relaxation protocol using none, half or full dose (1.0 mg) of oestradiol benzoate in Dorper ewes subjected to non-surgical embryo recovery (NSER). Thirty-six pluriparous ewes received progestogen sponge (60 mg) for 9 days plus eCG administration (300 IU i.m.) 24 hr before sponge removal. Ewes were not mated and were randomly assigned to receive at 16 hr before NSER 37.5 µg d-cloprostenol i.m. and different doses of oestradiol benzoate: 0.0 mg (0EB group; n = 12); 0.5 mg (0.5EB group; n = 12) or 1.0 mg of oestradiol (1.0EB group, n = 12). All ewes received oxytocin (50 IU) i.v. 20 min before NSER, which was performed 8 days after sponge removal. Corpora lutea were counted by transrectal ultrasonography 24 hr before NSER. After procedure, the ewes were kept in natural breeding period to check their post-NSER fertility. NSER was performed in 91.7% (33/36) of the animals with overall fluid recovery efficiency over 97% (p > .05). The cervical transposing with Hegar dilator was longer (p < .05) in 0EB (4.2 ± 0.3 min) compared to 0.5EB (1.7 ± 0.3 min) and 1.0EB group (1.5 ± 0.3 min). The cervical transposing with mandrel/catheter was longer (p < .05) in 0EB (2.4 ± 0.5 min) than 1.0EB group (1.3 ± 0.5 min). Overall duration of uterine flushing was 25.4 min with structure recovery rate of 43.5%, with no difference among groups (p > .05). The post-NSER fertility was higher (p < .05) in 0.0EB (90%) than 0.5EB group (36.4%). In conclusion, NSER can be successfully performed in Dorper ewes by using a cervical relaxation protocol without oestradiol benzoate.
Asunto(s)
Estradiol/análogos & derivados , Oveja Doméstica , Recolección de Tejidos y Órganos/veterinaria , Animales , Cuello del Útero/efectos de los fármacos , Transferencia de Embrión/métodos , Transferencia de Embrión/veterinaria , Embrión de Mamíferos , Estradiol/farmacología , Sincronización del Estro , Femenino , Fertilidad , Recolección de Tejidos y Órganos/métodosRESUMEN
Conjugated linoleic acid (CLA) is a mixture of positional isomers of linoleic acid found in meat and dairy products from ruminants. It is a trans fat widely used by athletes as a food supplement, due to a supposed effect of maximizing the use of body fat reserves. The interest in diet and culture media supplementation with CLA is an emerging area, demanding studies in order to elucidate its benefits in the reproductive parameters, as well as in cryopreservation. Therefore, the aim of this review was to discuss the effects of CLA on the oocytes, sperm and embryos cryotolerance. Some studies have already demonstrated its use in cryopreservation of germline. Among those, it was observed that CLA supplementation during oocyte in vitro maturation can increase their viability post-freezing and developmental capacity. Regarding the use of CLA on sperm, there are few studies and their results are still inconclusive. Finally, studies about CLA supplementation on embryo culture media have shown promising results, indicating that this bioactive molecule is able to modulate lipid uptake on blastomeres. Altogether, these findings demonstrate the potential use of CLA as a bioactive molecule to improve germline and embryo cryotolerance and open new perspectives on human and animal reproduction field.
O ácido linoleico conjugado (CLA) é uma mistura de isômeros posicionais do ácido linoleico encontrado em carne e laticínios de ruminantes. É um tipo de gordura trans muito utilizada por atletas para como suplemento alimentar devido a um suposto efeito de maximizar a utilização das reservas de gordura corporal. O interesse na suplementação de dietas e meios de cultura com o CLA é uma área emergente, exigindo estudos para elucidar seus benefícios nos parâmetros reprodutivos e na criopreservação. Dessa forma, o objetivo dessa revisão foi discutir os efeitos do CLA na criotolerância de oócitos, espermatozóides e embriões. Alguns estudos já demonstraram seu uso na criopreservação da linhagem germinativa. Entre esses, foi observado que a suplementação de CLA durante a maturação in vitro de oócitos pode aumentar sua viabilidade pós-congelamento e capacidade de desenvolvimento. Em relação ao uso de CLA no esperma, existem poucos estudos e seus resultados ainda são inconclusivos. Por último, estudos sobre a suplementação de CLA em meios de cultura de embriões mostraram resultados promissores, indicando que essa molécula bioativa é capaz de modular a captação de lipídios em blastômeros. No total, essas descobertas demonstram o potencial uso do CLA como uma molécula bioativa para melhorar a linha germinativa e a criotolerância ao embrião e abrir novas perspectivas no campo da reprodução humana e animal.
Asunto(s)
Animales , Embrión de Mamíferos , Espermatozoides , Oocitos , Respuesta al Choque por Frío/fisiología , Ácidos Linoleicos Conjugados/uso terapéutico , Criopreservación/veterinaria , Suplementos DietéticosRESUMEN
The objective of this study was to evaluate the effects of dietary chromium supplementation on hepatic gene expression of lactating Girolando (Holstein x Gyr) cows under heat stress conditions in climatic chamber. Thirty-six ¾ Holstein x Gyr lactating cows were used, based on a 2x3 factorial scheme, to evaluate the effects of two diets (0 vs 0.50 mg of organic chromium kg-¹ dry matter) and three environmental conditions (ECs): heat stress conditions in climatic chamber with ad libitum feeding (HS), a thermoneutral environment with ad libitum feeding (TN), and a pair-fed group in a thermoneutral environment (PF). Under HS group, the expression levels of glucose transporter 2(GLUT2), glucose-6-phosphatase (G6Pase), and growth hormone receptor (rGH) were down regulated (P < 0.05) in chromium-supplemented cows compared to those in cows fed the control diet. GLUT2 expression was upregulated (P = 0.02) in the HS group and insulin-like growth factor 1 (IGF1) was downregulated (P < 0.01) in the PF group in cows fed the control diet compared to the expressionin the TN group. No differences were observed between the ECs in terms of relative abundances of GLUT2, phosphoenolpyruvate carboxykinase (PEPCK), G6Pase, rGH, and IGF1 transcripts among the chromium-supplemented cows (P > 0.05). Heat stress caused changes in the expression of genes related to glucose metabolism, and organic chromium could modulate glucose metabolism in animals under heat stress conditions to some extent.(AU)
O objetivo deste estudo foi avaliar o efeito da suplementação com cromo na dieta na expressão gênica hepática de vacas Girolando (Holstein x Gyr) sob estresse térmico pelo calor em câmara climática. Foram utilizadas 36 vacas da raça Holandês x Gir, em um esquema fatorial 2x3, para avaliar duas dietas (0 vs 0,50 mg de cromo orgânico kg-1 de matéria seca) e três condições ambientais: condições de estresse térmico pelo calor em câmara climática com alimentação ad libitum (HS), ambiente termoneutro com alimentação ad libitum (TN) e um grupo com alimentação restrita em um ambiente termoneutro (PF). No grupo HS, as expressões de transportador de glicose 2 (GLUT2), glicose-6-fosfatase (G6Pase) e receptor de hormônio de crescimento (rGH) foram reguladas negativamente (P < 0,05) nas vacas suplementadas com cromo orgânico em comparação com as vacas alimentadas com a dieta controle. A expressão de GLUT2 foi regulada positivamente (P < 0,02) no grupo HS e o fator de crescimento semelhante à insulina 1 (IGF1) foi regulado negativamente (P < 0,01) no grupo PF em comparação como grupo TN para as vacas alimentadas com a dieta controle. Não foram observadas diferenças entre as diferentes condições ambientais na abundância relativa de GLUT2, fosfoenolpiruvato carboxiquinase (PEPCK), G6Pase, rGH e transcritos de IGF1 para as vacas suplementadas com cromo orgânico(P > 0.05). O estresse térmico pelo calor causou alterações na expressão de genes relacionados ao metabolismo da glicose, e o cromo orgânico pode modular o metabolismo da glicose em animais sob essas condições de estresse pelo calor.(AU)
Asunto(s)
Animales , Femenino , Bovinos , Bovinos/metabolismo , Dieta/veterinaria , Cromo/administración & dosificación , Cromo/efectos adversos , Respuesta al Choque Térmico , Hepatopatías/veterinariaRESUMEN
The objective of this study was to evaluate the effects of dietary chromium supplementation on hepatic gene expression of lactating Girolando (Holstein x Gyr) cows under heat stress conditions in climatic chamber. Thirty-six ¾ Holstein x Gyr lactating cows were used, based on a 2x3 factorial scheme, to evaluate the effects of two diets (0 vs 0.50 mg of organic chromium kg-¹ dry matter) and three environmental conditions (ECs): heat stress conditions in climatic chamber with ad libitum feeding (HS), a thermoneutral environment with ad libitum feeding (TN), and a pair-fed group in a thermoneutral environment (PF). Under HS group, the expression levels of glucose transporter 2(GLUT2), glucose-6-phosphatase (G6Pase), and growth hormone receptor (rGH) were down regulated (P 0.05). Heat stress caused changes in the expression of genes related to glucose metabolism, and organic chromium could modulate glucose metabolism in animals under heat stress conditions to some extent.
O objetivo deste estudo foi avaliar o efeito da suplementação com cromo na dieta na expressão gênica hepática de vacas Girolando (Holstein x Gyr) sob estresse térmico pelo calor em câmara climática. Foram utilizadas 36 vacas da raça Holandês x Gir, em um esquema fatorial 2x3, para avaliar duas dietas (0 vs 0,50 mg de cromo orgânico kg-1 de matéria seca) e três condições ambientais: condições de estresse térmico pelo calor em câmara climática com alimentação ad libitum (HS), ambiente termoneutro com alimentação ad libitum (TN) e um grupo com alimentação restrita em um ambiente termoneutro (PF). No grupo HS, as expressões de transportador de glicose 2 (GLUT2), glicose-6-fosfatase (G6Pase) e receptor de hormônio de crescimento (rGH) foram reguladas negativamente (P 0.05). O estresse térmico pelo calor causou alterações na expressão de genes relacionados ao metabolismo da glicose, e o cromo orgânico pode modular o metabolismo da glicose em animais sob essas condições de estresse pelo calor.
Asunto(s)
Femenino , Animales , Bovinos , Bovinos/metabolismo , Cromo/administración & dosificación , Cromo/efectos adversos , Dieta/veterinaria , Hepatopatías/veterinaria , Respuesta al Choque TérmicoRESUMEN
Background: Sperm capacitation is a process consists of a series of functional, biochemical, and biophysical modificationsthat render the ejaculated sperm competent for oocyte fertilization. Secreted by the female reproductive tract epithelium,heparin promotes capacitation by binding to and removing seminal plasma proteins, which are adsorbed to the sperm PMand would inhibit capacitation. There is substantial evidence that cryopreservation promotes capacitation-like changes inbull, ram and buck sperm. Our general hypotheses were: (a) cryopreserved ram sperm suffer capacitation more quicklythan buck and bull sperm under the same conditions; (b) the capacitation status of ruminant cryopreserved sperm is similarwhether or not heparin is present after the mini-Percoll technique; and (c) ruminant frozen-thawed sperm selected by miniPercoll and incubated within media without heparin supplementation is not impaired in terms of capacitation status andsperm agglutination. This study aimed to compare sperm parameters of ovine, caprine, and bovine frozen-thawed spermafter mini-Percoll processing followed by incubation with or without heparin supplementation.Materials, Methods & Results: Commercial semen of all species were used. Sperm samples were selected by mini-Percolland supplemented (or not) with heparin within an incubation medium for 18 h. Sperm kinematics (CASA system analyzes),capacitation status (CTC staining) and sperm agglutination were evaluated after thawing, mini-Percoll, 1.5 h, 3 h, 6 h and18 h. In comparison with post-thawing analysis, ovine species demonstrated a reduction (P < 0.05) in most of the spermmotility parameters after mini-Percoll. Conversely, ovine samples presented...(AU)
Asunto(s)
Animales , Masculino , Bovinos , Ovinos , Rumiantes , Espermatozoides/ultraestructura , Heparina , Capacitación Espermática , Criopreservación/veterinariaRESUMEN
We used a goat as a live incubator, along with associated nonsurgical embryo transfer techniques, to perform ex situ (in vivo) maturation of bovine oocytes. Immature bovine cumulus-oocyte complexes (COCs) aspirated from 3-8 mm follicles from slaughterhouse ovaries were randomly split into two groups for in vitro (IVM; n = 38) and ex situ maturation (ESM; n = 40). IVM was performed for a period of 24 h at 38.5 ºC and with 5% CO2 in the air of maximum humidity. For ESM, a presynchronized nulliparous goat (12 months old) received 40 immature COCs in the uterine horn apiece, via the transcervical route. After 24 h the structures were retrieved through uterine flushing. Analyses of nuclear maturation and lipid quantification were performed on oocytes from both groups. Fluorescent intensity was compared using the Studentâs t-test. Forty-seven percent of the structures were recovered after uterine flushing (19/40). The nuclear maturation rate was 94.5% (18/19) and 81.6% (31/38) for the ESM and IVM groups, respectively. In vitro-matured COCs contained more lipid droplets, expressed as a higher amount (p < 0.05) of emitted fluorescent light than ex situ-matured COCs (858 ± 73 vs. 550 ± 64 arbitrary fluorescence units, respectively). This is the first report to associate nonsurgical embryo transfer techniques and a goat as a live incubator for the maturation of bovine oocytes. We
Utilizamos uma cabra como incubadora viva, juntamente com técnicas de transferência de embriões não cirúrgicas associadas, para realizar a maturação ex situ (in vivo) de oócitos bovinos. Os complexos cumulus-oócitos bovinos (COCs), aspirados de folÃculos de 3-8 mm de ovários de abatedouro foram aleatoriamente divididos em dois grupos para maturação in vitro (IVM; n = 38) e ex situ (ESM; n = 40). A MIV foi realizada por um perÃodo de 24 h no meio TCM-199, a 38,5 ºC, e com 5% de CO2 em umidade máxima. Para o ESM, uma cabra nulÃpara pré-sincronizada (12 meses de idade) recebeu 40 COCs imaturos no ápice do corno uterino, por via transcervical. Após 24 h as estruturas foram recuperadas através de lavagem uterina. Análises de maturação nuclear e quantificação de lipÃdios foram realizadas em oócitos de ambos os grupos. A intensidade de fluorescente foi comparada usando o teste t de Student. Quarenta e sete por cento das estruturas foram recuperadas após lavagem uterina (19/40). A taxa de maturação nuclear foi de 94,5% (18/19) e 81,6% (31/38) para os grupos ESM e IVM, respectivamente. Os COCs maturados in vitro continham mais gotÃculas lipÃdicas, expressos como uma quantidade maior (p < 0,05) da luz fluorescente emitida do que os COCs ex situ (858 ± 73 vs 550 ± 64 unidades de fluorescência arbitrárias, respectivamente). Este é o primeiro relató
RESUMEN
A obtenção de oócitos de boa qualidade é essencial para o sucesso de diversas biotécnicas reprodutivas. Objetivou-se determinar o efeito de duas técnicas na recuperação de oócitos de boa qualidade em gatas e cadelas em diferentes estágios reprodutivos. Foram utilizados 43 pares de ovários de gata e 35 de cadela após realização da ovariosalpingohisterectomia eletiva. A fase do ciclo estral foi classificada em inativa, folicular ou luteal. Os ovários da fase folicular foram divididos em três grupos: PUN) punção dos folículos com agulha; PUN+FAT) fatiamento do mesmo ovário já puncionado; e FAT) fatiamento do segundo ovário. Os ovários das fêmeas em fase luteal e inativa foram submetidos ao FAT. Foram obtidos no total 974 oócitos (~23/animal) nas fêmeas felinas e 940 (~27/animal) nas caninas. O fatiamento recuperou número superior (P<0,05) de oócitos. Não houve diferença (P>0,05) entre as técnicas de coleta na qualidade de estruturas recuperadas. A quantidade de oócitos recuperados em cada fase foi similar (P>0,05). Contudo, a fase inativa foi superior à luteal (P<0,05) e semelhante à folicular na quantidade de oócitos de boa qualidade em gatas e não houve diferença em cadelas. Conclui-se que o fatiamento recupera maior quantidade de oócitos, não influenciando em sua qualidade. As fases inativa e folicular recuperam maior quantidade de oócitos de boa qualidade em gatas e não afetam a recuperação em cadelas. Portanto, para otimizar o uso das biotecnologias, deve-se levar em consideração o estágio do ciclo estral em fêmeas felinas e a técnica de coleta utilizada na recuperação de oócitos.(AU)
The recovery of good quality oocytes is essential for the success of various reproductive biotechniques. The aim of this study was to determine the effect of two techniques on the recovery of good quality oocytes in queens and bitches at different reproductive stages. A total of 43 pairs of ovaries of queens and 35 of bitches after elective ovariosalpingohisterectomy were performed. The estrous cycle phase was classified as inactive, follicular or luteal. The ovaries of the follicular phase were allocated into three groups: PUN) puncture of the follicles with a needle; PUN + SLI) slicing of the same ovary already punctured; and SLI) slicing of the second ovary. The ovaries of luteal and inactive females were submitted to SLI. A total of 974 oocytes (~23/animal) were obtained in feline females and 940 (~27/animal) in canines females. The SLI technique recovered superior number (P<0.05) of oocytes. There was no difference (P>0.05) between the collection techniques in the quality of recovered structures. The number of oocytes recovered in each phase was similar (P>0.05). However, the inactive phase was higher than luteal (P<0.05) and similar to the follicular phase in the quantity of good-quality oocytes in queens and there was no difference in bitches. In conclusion, it is preferable to perform the slicing technique to recover more oocytes in both species. Moreover, in queens it is possible to obtain good quality oocytes in the inactive phase and in bitches the estrous cycle phase does not influence the quality.(AU)
Asunto(s)
Animales , Femenino , Gatos , Perros , Recuperación del Oocito/métodos , Recuperación del Oocito/veterinaria , Ciclo Estral , BiotecnologíaRESUMEN
This study investigated the feasibility of applying fixed-time (cryopreserved) embryo transfer in ewes. Embryos (n = 106) were non-surgically recovered from superovulated donors (n = 39) on day 6-7 after oestrus. Straws containing one or two embryos (morulae and/or blastocysts) subjected to either slow freezing (SF, n = 62) or vitrification (VT, n = 44) were randomly used within fixed-time embryo transfer on Day 8.5. Recipient ewes were nulliparous (n = 58) bearing corpora lutea after synchronous oestrous induction protocol. The pregnancy rate was higher (p = .03) in SF (39.4%) than VT (16.9%) and survival rate tended (p = .08) to be higher in SF than in VT (25.8% vs. 15.9%). Lambing rates were similar (p = .13) between SF (20.9%) and VT (15.9%). Embryos recovered by non-surgical route after cervical dilation treatment and later cryopreserved by either slow freezing or vitrification produced reasonable pregnancy rates after FTET.
Asunto(s)
Criopreservación/veterinaria , Transferencia de Embrión/veterinaria , Índice de Embarazo , Animales , Tasa de Natalidad , Blastocisto , Criopreservación/métodos , Femenino , Congelación , Mórula , Embarazo , Oveja Doméstica , VitrificaciónRESUMEN
A obtenção de oócitos de boa qualidade é essencial para o sucesso de diversas biotécnicas reprodutivas. Objetivou-se determinar o efeito de duas técnicas na recuperação de oócitos de boa qualidade em gatas e cadelas em diferentes estágios reprodutivos. Foram utilizados 43 pares de ovários de gata e 35 de cadela após realização da ovariosalpingohisterectomia eletiva. A fase do ciclo estral foi classificada em inativa, folicular ou luteal. Os ovários da fase folicular foram divididos em três grupos: PUN) punção dos folículos com agulha; PUN+FAT) fatiamento do mesmo ovário já puncionado; e FAT) fatiamento do segundo ovário. Os ovários das fêmeas em fase luteal e inativa foram submetidos ao FAT. Foram obtidos no total 974 oócitos (~23/animal) nas fêmeas felinas e 940 (~27/animal) nas caninas. O fatiamento recuperou número superior (P<0,05) de oócitos. Não houve diferença (P>0,05) entre as técnicas de coleta na qualidade de estruturas recuperadas. A quantidade de oócitos recuperados em cada fase foi similar (P>0,05). Contudo, a fase inativa foi superior à luteal (P<0,05) e semelhante à folicular na quantidade de oócitos de boa qualidade em gatas e não houve diferença em cadelas. Conclui-se que o fatiamento recupera maior quantidade de oócitos, não influenciando em sua qualidade. As fases inativa e folicular recuperam maior quantidade de oócitos de boa qualidade em gatas e não afetam a recuperação em cadelas. Portanto, para otimizar o uso das biotecnologias, deve-se levar em consideração o estágio do ciclo estral em fêmeas felinas e a técnica de coleta utilizada na recuperação de oócitos.
The recovery of good quality oocytes is essential for the success of various reproductive biotechniques. The aim of this study was to determine the effect of two techniques on the recovery of good quality oocytes in queens and bitches at different reproductive stages. A total of 43 pairs of ovaries of queens and 35 of bitches after elective ovariosalpingohisterectomy were performed. The estrous cycle phase was classified as inactive, follicular or luteal. The ovaries of the follicular phase were allocated into three groups: PUN) puncture of the follicles with a needle; PUN + SLI) slicing of the same ovary already punctured; and SLI) slicing of the second ovary. The ovaries of luteal and inactive females were submitted to SLI. A total of 974 oocytes (~23/animal) were obtained in feline females and 940 (~27/animal) in canines females. The SLI technique recovered superior number (P<0.05) of oocytes. There was no difference (P>0.05) between the collection techniques in the quality of recovered structures. The number of oocytes recovered in each phase was similar (P>0.05). However, the inactive phase was higher than luteal (P<0.05) and similar to the follicular phase in the quantity of good-quality oocytes in queens and there was no difference in bitches. In conclusion, it is preferable to perform the slicing technique to recover more oocytes in both species. Moreover, in queens it is possible to obtain good quality oocytes in the inactive phase and in bitches the estrous cycle phase does not influence the quality.
Asunto(s)
Animales , Gatos , Perros , Oocitos , Gatos/anatomía & histología , Técnicas Reproductivas/veterinaria , Ciclo Estral , Perros/anatomía & histología , Recuperación del Oocito/veterinaria , Ovario , Fase Folicular , Fase LuteínicaRESUMEN
A obtenção de oócitos de boa qualidade é essencial para o sucesso de diversas biotécnicas reprodutivas. Objetivou-se determinar o efeito de duas técnicas na recuperação de oócitos de boa qualidade em gatas e cadelas em diferentes estágios reprodutivos. Foram utilizados 43 pares de ovários de gata e 35 de cadela após realização da ovariosalpingohisterectomia eletiva. A fase do ciclo estral foi classificada em inativa, folicular ou luteal. Os ovários da fase folicular foram divididos em três grupos: PUN) punção dos folículos com agulha; PUN+FAT) fatiamento do mesmo ovário já puncionado; e FAT) fatiamento do segundo ovário. Os ovários das fêmeas em fase luteal e inativa foram submetidos ao FAT. Foram obtidos no total 974 oócitos (~23/animal) nas fêmeas felinas e 940 (~27/animal) nas caninas. O fatiamento recuperou número superior (P0,05) entre as técnicas de coleta na qualidade de estruturas recuperadas. A quantidade de oócitos recuperados em cada fase foi similar (P>0,05). Contudo, a fase inativa foi superior à luteal (P<0,05) e semelhante à folicular na quantidade de oócitos de boa qualidade em gatas e não houve diferença em cadelas. Conclui-se que o fatiamento recupera maior quantidade de oócitos, não influenciando em sua qualidade. As fases inativa e folicular recuperam maior quantidade de oócitos de boa qualidade em gatas e não afetam a recuperação em cadelas. Portanto, para otimizar o uso das biotecnologias, deve-se levar em consideração o estágio do ciclo estral em fêmeas felinas e a técnica de coleta utilizada na recuperação de oócitos.
The recovery of good quality oocytes is essential for the success of various reproductive biotechniques. The aim of this study was to determine the effect of two techniques on the recovery of good quality oocytes in queens and bitches at different reproductive stages. A total of 43 pairs of ovaries of queens and 35 of bitches after elective ovariosalpingohisterectomy were performed. The estrous cycle phase was classified as inactive, follicular or luteal. The ovaries of the follicular phase were allocated into three groups: PUN) puncture of the follicles with a needle; PUN + SLI) slicing of the same ovary already punctured; and SLI) slicing of the second ovary. The ovaries of luteal and inactive females were submitted to SLI. A total of 974 oocytes (~23/animal) were obtained in feline females and 940 (~27/animal) in canines females. The SLI technique recovered superior number (P0.05) between the collection techniques in the quality of recovered structures. The number of oocytes recovered in each phase was similar (P>0.05). However, the inactive phase was higher than luteal (P<0.05) and similar to the follicular phase in the quantity of good-quality oocytes in queens and there was no difference in bitches. In conclusion, it is preferable to perform the slicing technique to recover more oocytes in both species. Moreover, in queens it is possible to obtain good quality oocytes in the inactive phase and in bitches the estrous cycle phase does not influence the quality.
Asunto(s)
Femenino , Animales , Gatos , Perros , Ciclo Estral , Recuperación del Oocito/métodos , Recuperación del Oocito/veterinaria , BiotecnologíaRESUMEN
We used a goat as a live incubator, along with associated nonsurgical embryo transfer techniques, to perform ex situ (in vivo) maturation of bovine oocytes. Immature bovine cumulus-oocyte complexes (COCs) aspirated from 3-8 mm follicles from slaughterhouse ovaries were randomly split into two groups for in vitro (IVM; n = 38) and ex situ maturation (ESM; n = 40). IVM was performed for a period of 24 h at 38.5 ºC and with 5% CO2 in the air of maximum humidity. For ESM, a presynchronized nulliparous goat (12 months old) received 40 immature COCs in the uterine horn apiece, via the transcervical route. After 24 h the structures were retrieved through uterine flushing. Analyses of nuclear maturation and lipid quantification were performed on oocytes from both groups. Fluorescent intensity was compared using the Studentâs t-test. Forty-seven percent of the structures were recovered after uterine flushing (19/40). The nuclear maturation rate was 94.5% (18/19) and 81.6% (31/38) for the ESM and IVM groups, respectively. In vitro-matured COCs contained more lipid droplets, expressed as a higher amount (p < 0.05) of emitted fluorescent light than ex situ-matured COCs (858 ± 73 vs. 550 ± 64 arbitrary fluorescence units, respectively). This is the first report to associate nonsurgical embryo transfer techniques and a goat as a live incubator for the maturation of bovine oocytes. We
Utilizamos uma cabra como incubadora viva, juntamente com técnicas de transferência de embriões não cirúrgicas associadas, para realizar a maturação ex situ (in vivo) de oócitos bovinos. Os complexos cumulus-oócitos bovinos (COCs), aspirados de folÃculos de 3-8 mm de ovários de abatedouro foram aleatoriamente divididos em dois grupos para maturação in vitro (IVM; n = 38) e ex situ (ESM; n = 40). A MIV foi realizada por um perÃodo de 24 h no meio TCM-199, a 38,5 ºC, e com 5% de CO2 em umidade máxima. Para o ESM, uma cabra nulÃpara pré-sincronizada (12 meses de idade) recebeu 40 COCs imaturos no ápice do corno uterino, por via transcervical. Após 24 h as estruturas foram recuperadas através de lavagem uterina. Análises de maturação nuclear e quantificação de lipÃdios foram realizadas em oócitos de ambos os grupos. A intensidade de fluorescente foi comparada usando o teste t de Student. Quarenta e sete por cento das estruturas foram recuperadas após lavagem uterina (19/40). A taxa de maturação nuclear foi de 94,5% (18/19) e 81,6% (31/38) para os grupos ESM e IVM, respectivamente. Os COCs maturados in vitro continham mais gotÃculas lipÃdicas, expressos como uma quantidade maior (p < 0,05) da luz fluorescente emitida do que os COCs ex situ (858 ± 73 vs 550 ± 64 unidades de fluorescência arbitrárias, respectivamente). Este é o primeiro relató
RESUMEN
We used a goat as a live incubator, along with associated nonsurgical embryo transfer techniques, to perform ex situ (in vivo) maturation of bovine oocytes. Immature bovine cumulus-oocyte complexes (COCs) aspirated from 3-8 mm follicles from slaughterhouse ovaries were randomly split into two groups for in vitro (IVM; n = 38) and ex situ maturation (ESM; n = 40). IVM was performed for a period of 24 h at 38.5 ºC and with 5% CO2 in the air of maximum humidity. For ESM, a presynchronized nulliparous goat (12 months old) received 40 immature COCs in the uterine horn apiece, via the transcervical route. After 24 h the structures were retrieved through uterine flushing. Analyses of nuclear maturation and lipid quantification were performed on oocytes from both groups. Fluorescent intensity was compared using the Studentâs t-test. Forty-seven percent of the structures were recovered after uterine flushing (19/40). The nuclear maturation rate was 94.5% (18/19) and 81.6% (31/38) for the ESM and IVM groups, respectively. In vitro-matured COCs contained more lipid droplets, expressed as a higher amount (p < 0.05) of emitted fluorescent light than ex situ-matured COCs (858 ± 73 vs. 550 ± 64 arbitrary fluorescence units, respectively). This is the first report to associate nonsurgical embryo transfer techniques and a goat as a live incubator for the maturation of bovine oocytes. We
Utilizamos uma cabra como incubadora viva, juntamente com técnicas de transferência de embriões não cirúrgicas associadas, para realizar a maturação ex situ (in vivo) de oócitos bovinos. Os complexos cumulus-oócitos bovinos (COCs), aspirados de folÃculos de 3-8 mm de ovários de abatedouro foram aleatoriamente divididos em dois grupos para maturação in vitro (IVM; n = 38) e ex situ (ESM; n = 40). A MIV foi realizada por um perÃodo de 24 h no meio TCM-199, a 38,5 ºC, e com 5% de CO2 em umidade máxima. Para o ESM, uma cabra nulÃpara pré-sincronizada (12 meses de idade) recebeu 40 COCs imaturos no ápice do corno uterino, por via transcervical. Após 24 h as estruturas foram recuperadas através de lavagem uterina. Análises de maturação nuclear e quantificação de lipÃdios foram realizadas em oócitos de ambos os grupos. A intensidade de fluorescente foi comparada usando o teste t de Student. Quarenta e sete por cento das estruturas foram recuperadas após lavagem uterina (19/40). A taxa de maturação nuclear foi de 94,5% (18/19) e 81,6% (31/38) para os grupos ESM e IVM, respectivamente. Os COCs maturados in vitro continham mais gotÃculas lipÃdicas, expressos como uma quantidade maior (p < 0,05) da luz fluorescente emitida do que os COCs ex situ (858 ± 73 vs 550 ± 64 unidades de fluorescência arbitrárias, respectivamente). Este é o primeiro relató
RESUMEN
Background: Sperm capacitation is a process consists of a series of functional, biochemical, and biophysical modificationsthat render the ejaculated sperm competent for oocyte fertilization. Secreted by the female reproductive tract epithelium,heparin promotes capacitation by binding to and removing seminal plasma proteins, which are adsorbed to the sperm PMand would inhibit capacitation. There is substantial evidence that cryopreservation promotes capacitation-like changes inbull, ram and buck sperm. Our general hypotheses were: (a) cryopreserved ram sperm suffer capacitation more quicklythan buck and bull sperm under the same conditions; (b) the capacitation status of ruminant cryopreserved sperm is similarwhether or not heparin is present after the mini-Percoll technique; and (c) ruminant frozen-thawed sperm selected by miniPercoll and incubated within media without heparin supplementation is not impaired in terms of capacitation status andsperm agglutination. This study aimed to compare sperm parameters of ovine, caprine, and bovine frozen-thawed spermafter mini-Percoll processing followed by incubation with or without heparin supplementation.Materials, Methods & Results: Commercial semen of all species were used. Sperm samples were selected by mini-Percolland supplemented (or not) with heparin within an incubation medium for 18 h. Sperm kinematics (CASA system analyzes),capacitation status (CTC staining) and sperm agglutination were evaluated after thawing, mini-Percoll, 1.5 h, 3 h, 6 h and18 h. In comparison with post-thawing analysis, ovine species demonstrated a reduction (P < 0.05) in most of the spermmotility parameters after mini-Percoll. Conversely, ovine samples presented...
Asunto(s)
Masculino , Animales , Bovinos , Capacitación Espermática , Espermatozoides/ultraestructura , Heparina , Ovinos , Rumiantes , Criopreservación/veterinariaRESUMEN
A presente revisão tem por objetivo abordar os aspectos técnicos em estudos nas diferentes etapas damúltipla ovulação e transferência de embriões em ovinos (MOTE). Apesar dos inúmeros avanços a altavariabilidade de resposta à superovulação ainda é um entrave para esta biotécnica. Visando driblar este gargalodiferentes estratégias têm sido testadas para selecionar fêmeas com melhor potencial de resposta, como acontagem de folículos antrais, pré-seleção com eCG, repetibilidade de resposta, dosagem do hormônio antiMüllerianoe sincronização da onda folicular. Ajustes de protocolos superovulatórios modificando a frequência,o número de aplicações e a diminuição da dose total de FSH, têm sido testados. Outra tendência é a substituiçãode procedimentos cirúrgicos por técnicas menos invasivas, prezando pelo bem estar animal e também pelasimplificação de processos. Resultados satisfatórios para avaliação de doadoras por ultrassonografia ao invés delaparoscopia ilustram esta tendência. Adicionalmente, a inovulação não cirúrgica já se mostra exequível. Porém,etapas como a seleção de receptoras e a criopreservação de embriões também têm potencial para melhorar osíndices. Associando os esforços e resultados de diferentes linhas de pesquisas, a MOTE em ovinos têm evoluídoe seu uso para pesquisa ou produção animal tem-se ampliado.(AU)
This review address technical aspects that are being studied in multiple ovulation and embryo transferin sheep (MOTE). Despite the numerous advances the high variability of response to superovulation still abarrier for this biotechnology. Aiming to suppress this limitation, different strategies have been tested to selectewes with high ovulatory response such as antral follicle count, pre-selection with eCG, repeatability ofresponse, anti-Müllerian hormone, and follicular wave synchronization. Adjustments of superovulatoryprotocols modifying the frequency, the number of applications and a decrease in the total FSH dose are alsobeing tested. Another trend is the replacement of surgical procedures for less invasive techniques, focusinganimal welfare and simplification of procedures. Satisfactory results using ultrasonography to evaluate donors,rather than laparoscopy illustrate this trend. Also non-surgical embryo transfer is already feasible in ewes.However, adjustments in recipients selection and embryo cryopreservation can potentially improve pregnancyrates. By linking the efforts and results of different lines of research, MOTE in sheep has improved and it is usefor research or animal production increased.(AU)