Analysis of physical traits, clinical parameters, and energy metabolism of in vivo- and in vitro-derived Flemish newborn calves during the first day of life.

Studies investigating physiological deviations from normality in newborn calves derived from in vitro fertilization procedures remain important for the understanding of factors that reduce calf survival after birth. The aim of this study was to investigate parameters affecting health and welfare of newborn Flemish calves derived from in vitro embryo production (IVP) in the first hours of life in comparison to in vivo-derived calves. Physical traits of newborn calves and fetal membranes (FM) were recorded soon after birth. Newborn venous blood samples were collected at several time points within the first 24 h of life for analyses of energy substrates, electrolytes, blood gases, acid-base balance, blood chemistry, and haematology. A liver biopsy was taken within the first hour after birth for analysis of gene expression of key enzymes of the fructolytic and glycolytic pathways. Newborn IVP calves were heavier and larger at birth, which was associated with heavier FM. At several time points during the first 24 h of life, IVP-derived calves had altered rectal temperature, blood gases, electrolyte concentrations, blood parameters for liver, kidney and muscle function, and acid-base balance, plasma lipid metabolism, and hemogram parameters. The relative mRNA abundances for triokinase and lactate dehydrogenase-B were greater in IVP calves. In summary, IVP-derived newborn calves were at higher risk of clinical problems after birth, which was markedly greater in heavier and larger calves. Such animals take longer to adapt to extrauterine life and should receive a special attention during the immediate neonatal period.

Expression profile of key genes involved in DNA repair mechanisms in bovine cumulus cells cultured with bovine serum albumin or fetal calf serum.

Cumulus cells from cumulus-oocyte complexes (COC) matured in vitro in serum-free medium show high incidence of apoptosis and DNA double-strand breaks (DSB). This study aimed to characterize the transcript expression profile of selected genes involved in DNA repair mechanisms in bovine cumulus cells cultured with bovine serum albumin (BSA) or fetal calf serum (FCS). Briefly, bovine cumulus-oocyte complexes were in vitro matured with either, 0.4% BSA or 10% FCS for 3, 6, 12 or 24 h. The total RNA of cumulus cells was used for real-time PCR analysis. Transcript abundance of XRCC6, XRCC5, DNAPK, GAAD45B, TP53BP1, RAD50, RAD52, ATM and BRCA2 target genes changed as the IVM proceeded (P < 0.05). However, an interaction between protein source (FCS or BSA) and time was not detected (P ≥ 0.05). Cumulus cells from COCs matured with BSA presented higher mRNA expression of two genes compared to FCS group: TP53BP1 at 6 h and BRCA1 at 3, 6, 12 and 24 h (P < 0.05). In summary, our results showed for the first time the expression profile of the key genes involved in DSB repair mechanisms in cumulus cells obtained from bovine COCs matured with FCS or BSA. The higher mRNA expression of BRCA1 and TP53BP1 and lower mRNA expression of TNFAIP6 suggests an increase in apoptosis rate and DNA damage in cumulus cells cultured in BSA-supplemented medium and may explain, at least to some extent, the reduced developmental potential of bovine oocytes matured in serum-free medium.

Porcine IVF embryo development and estrogen receptors are influenced by the concentration of percoll gradients during sperm selection.

This study aimed to evaluate the effect of three different concentrations of discontinuous gradients of percoll (90/45, 80/40, and 70/35) in the outcome of porcine in vitro fertilization (IVF) and its influence on further embryo development and quality. Embryo viability was assessed by the expression of estrogen receptors (E2 R) and cleaved caspase-3 (CC3). The highest percoll concentration (90/45) resulted in the lowest embryo production (24.9%) in comparison with 80/40 (37.5%) and 70/35 (40.0%), with the production being similar between the two lowest concentrations. The hatching rate for 90/45 (26.2%) was lower than for 80/40 (45.5%), and both were similar to the Group 70/35 (32.9%). The hatched embryos from the concentration 90/45 showed the lowest proportion of E2 R expression (3.6%), while the Groups 80/40 (22.6%) and 70/35 (39.3%) had a similar proportion of expression. The live embryos that did not hatch until Day 8 of culture presented a higher CC3 proportion for Group 90/45 (18.3%), in comparison with 80/40 (12.7%) and 70/35 (10.7%), with the latter two being similar. In conclusion, adjustments in percoll concentration used for sperm selection before porcine IVF can improve embryo production and competence for pregnancy recognition and establishment.

Vitrification of in vitro produced porcine blastocysts: influence of cryoprotectants toxicity and embryo age

Background: Porcine embryos are sensible to all assisted reproduction manipulations, especially the ones that involvecryopreservation. Despite the high cryoprotectant concentrations routinely applied, vitrification is the most effective technique to date. These substances toxicity can also play a negative role in embryo viability. During in vitro porcine embryoproduction, the speed of development is often unevenly distributed. It is possible that their development speed, affectsembryo tolerance to cryoprotectants. This study aimed to evaluate the toxicity of porcine embryos of days 5 or 6 of cultureto cryoprotectant agents; as well as to assess embryo survival to vitrification.Materials, Methods & Results: Parthenogenetic porcine blastocysts and expanded blastocysts of days 5 and 6 of culturewere exposed to toxicity tests (experiments 1 and 2) and vitrification (experiment 3) using different protocols. In the firstexperiment, three different cryoprotectants were used (Dimethyl sulfoxide - DMSO, Ethylene glycol - EG, and Sucrose- SUC), combined in three different associations (G1: 15% EG + 15% DMSO with 0.5 M SUC; G2: 16% EG + 16%DMSO with 0.4 M SUC; G3: 18% EG + 18% DMSO with 0.5 M SUC). In the fresh Control, embryos of day 6 are moresensible than the ones of day 5, whom showed a lower hatching rate (39.7 vs. 60.8%). After the toxicity (Experiment 1)test, the G1 showed better expansion rates in day 6 (50.0 vs 31.0 and 3.6% for G2 and G3) and higher hatching of day 6compared to G2 and G3 (23.2, vs. 8.6 and 0.0% for G2 and G3). The fresh non hatched embryos at day 8, derived at day6, had a lower percentage of cells with cleaved caspase-3 (20.2%) compared with the G1 (30.5%), G2 (31.4%) and G3(30.5%). The hatched embryos of day 5 from G2 had lower total cell number (TCN) compared with the day 6 hatchedembryos, whereas in G1 the TCN was not affected. The second experiment compared EG combined to one of these threeextracellular...(AU)

Superovulação em éguas da raça Crioula e Quarto de Milha com extrato de pituitária equina (EPE) / Superovulatory protocol with equine pituitary extract (EPE) in mares Crioula and the Quarter Horse

Este trabalho compara a resposta superovulatória de éguas doadoras de embriões das raças Quarto de Milha (QM) e Crioula, utilizando um protocolo com baixa dose de extrato de pituitária equina (EPE). Oito éguas QM e seis éguas Crioulas foram acompanhadas durante 3 ciclos estrais consecutivos, sendo que cada ciclo corresponde a um grupo. Grupo Controle monitoramento do crescimento folicular até a ovulação; Grupo EPE monitoramento ultrassonográfico até que os folículos atingissem cerca de 20 mm de diâmetro e, posteriormente, administração de 7 mg de EPE, duas vezes ao dia, até a indução da ovulação com 2500UI de hCG; Grupo Pós-EPE idem ao grupo controle. Os dados foram submetidos à análise de variância, utilizando o procedimento GLM do pacote estatístico SAS, sendo previamente testadas para normalidade dos resíduos, e as médias comparadas pelo teste de Tukey ao nível de 5%. Nas éguas Crioulas tratadas com EPE houve um aumento no número de ovulações (p=0,0534), com média de 3,33±2,06 quando comparadas aos grupos controle e pós-EPE e às éguas da raça QM (2,00±0,53). O tratamento com EPE na dose preconizada permitiu uma melhor resposta superovulatória e produção embrionária nas éguas Crioulas, quando comparadas com as éguas Quarto de Milha.(AU)

This study compared the superovulatory response of embryos donor mares of Quarter Horse (QH) and Crioula using a protocol with low dose of equine pituitary extract (EPE). Eight QH mares and six Crioula mares were monitored during 3 consecutive estrous cycles, with each cycle corresponds to a group. Control Group - monitoring of follicle growth up to the ovulation; EPE group - when the follicles reached 20 mm in diameter were administered 7 mg EPE twice daily. When the follicles achieved a diameter 35 mm, the ovulation was induced with 2500UI hCG; Post-EPE Group - idem to the control group. Data were analyzed using GLM procedure of the SAS statistical package. The variables were submitted to the Tukeys test and least square means adjusted for multiple comparisons using the Tukey-Kramers test, with significance level of 5%. Values are presented as mean ± SD. In the Crioula mares treated with EPE, there was an increase in the number of ovulations (p =0.0534) with a mean of 3.33 ± 2.06 ovulations when compared to the control and post-EPE groups, and mares QM. (2.00±0.53). Treatment with EPE in the recommended dose allowed better superovulatory response and rate of embryo recovery in Crioula mares when compared to the QM mares.(AU)

Superovulação em éguas da raça Crioula e Quarto de Milha com extrato de pituitária equina (EPE) / Superovulatory protocol with equine pituitary extract (EPE) in mares Crioula and the Quarter Horse

Este trabalho compara a resposta superovulatória de éguas doadoras de embriões das raças Quarto de Milha (QM) e Crioula, utilizando um protocolo com baixa dose de extrato de pituitária equina (EPE). Oito éguas QM e seis éguas Crioulas foram acompanhadas durante 3 ciclos estrais consecutivos, sendo que cada ciclo corresponde a um grupo. Grupo Controle – monitoramento do crescimento folicular até a ovulação; Grupo EPE – monitoramento ultrassonográfico até que os folículos atingissem cerca de 20 mm de diâmetro e, posteriormente, administração de 7 mg de EPE, duas vezes ao dia, até a indução da ovulação com 2500UI de hCG; Grupo Pós-EPE – idem ao grupo controle. Os dados foram submetidos à análise de variância, utilizando o procedimento GLM do pacote estatístico SAS, sendo previamente testadas para normalidade dos resíduos, e as médias comparadas pelo teste de Tukey ao nível de 5%. Nas éguas Crioulas tratadas com EPE houve um aumento no número de ovulações (p=0,0534), com média de 3,33±2,06 quando comparadas aos grupos controle e pós-EPE e às éguas da raça QM (2,00±0,53). O tratamento com EPE na dose preconizada permitiu uma melhor resposta superovulatória e produção embrionária nas éguas Crioulas, quando comparadas com as éguas Quarto de Milha.

This study compared the superovulatory response of embryos donor mares of Quarter Horse (QH) and Crioula using a protocol with low dose of equine pituitary extract (EPE). Eight QH mares and six Crioula mares were monitored during 3 consecutive estrous cycles, with each cycle corresponds to a group. Control Group - monitoring of follicle growth up to the ovulation; EPE group - when the follicles reached 20 mm in diameter were administered 7 mg EPE twice daily. When the follicles achieved a diameter 35 mm, the ovulation was induced with 2500UI hCG; Post-EPE Group - idem to the control group. Data were analyzed using GLM procedure of the SAS statistical package. The variables were submitted to the Tukey’s test and least square means adjusted for multiple comparisons using the Tukey-Kramer’s test, with significance level of 5%. Values are presented as mean ± SD. In the Crioula mares treated with EPE, there was an increase in the number of ovulations (p =0.0534) with a mean of 3.33 ± 2.06 ovulations when compared to the control and post-EPE groups, and mares QM. (2.00±0.53). Treatment with EPE in the recommended dose allowed better superovulatory response and rate of embryo recovery in Crioula mares when compared to the QM mares.

Vitrification of in vitro produced porcine blastocysts: influence of cryoprotectants toxicity and embryo age

Background: Porcine embryos are sensible to all assisted reproduction manipulations, especially the ones that involvecryopreservation. Despite the high cryoprotectant concentrations routinely applied, vitrification is the most effective technique to date. These substances toxicity can also play a negative role in embryo viability. During in vitro porcine embryoproduction, the speed of development is often unevenly distributed. It is possible that their development speed, affectsembryo tolerance to cryoprotectants. This study aimed to evaluate the toxicity of porcine embryos of days 5 or 6 of cultureto cryoprotectant agents; as well as to assess embryo survival to vitrification.Materials, Methods & Results: Parthenogenetic porcine blastocysts and expanded blastocysts of days 5 and 6 of culturewere exposed to toxicity tests (experiments 1 and 2) and vitrification (experiment 3) using different protocols. In the firstexperiment, three different cryoprotectants were used (Dimethyl sulfoxide - DMSO, Ethylene glycol - EG, and Sucrose- SUC), combined in three different associations (G1: 15% EG + 15% DMSO with 0.5 M SUC; G2: 16% EG + 16%DMSO with 0.4 M SUC; G3: 18% EG + 18% DMSO with 0.5 M SUC). In the fresh Control, embryos of day 6 are moresensible than the ones of day 5, whom showed a lower hatching rate (39.7 vs. 60.8%). After the toxicity (Experiment 1)test, the G1 showed better expansion rates in day 6 (50.0 vs 31.0 and 3.6% for G2 and G3) and higher hatching of day 6compared to G2 and G3 (23.2, vs. 8.6 and 0.0% for G2 and G3). The fresh non hatched embryos at day 8, derived at day6, had a lower percentage of cells with cleaved caspase-3 (20.2%) compared with the G1 (30.5%), G2 (31.4%) and G3(30.5%). The hatched embryos of day 5 from G2 had lower total cell number (TCN) compared with the day 6 hatchedembryos, whereas in G1 the TCN was not affected. The second experiment compared EG combined to one of these threeextracellular...

Células fetais bovinas de cultivo primário submetidas a diferentes pressões negativas antes do congelamento em palhetas / Fetal bovine primary culture cells submitted to different negative pressures before straw freezing

O congelamento de células é uma importante ferramenta na preservação de espécies ameaçadas de extinção. Células fetais de cultivo primário obtidas de um bovino clone foram submetidas à pressão negativa (PN) de 200, 500 ou 800 mbar, imediatamente (PN0h) ou três horas antes (PN3h) do congelamento em palhetas finas, com 10% de DMSO como crioprotetor. Células frescas e congeladas sem submissão à PN foram utilizadas como controles. Avaliou-se a viabilidade pós-descongelamento, a curva de proliferação celular, assim como o tempo de duplicação da população (PDT) celular, a cada 24 horas, durante oito dias. Os dados obtidos foram submetidos ao teste de Tukey ou Qui quadrado (P≤0,05). A sobrevivência média dos grupos controle (89,8%) e PN500 0h (88,1%) foi superior aos outros grupos; o tempo de PDT foi semelhante nos grupos fresco (27,5 ± 0,35 h), controle congelado (30,1 ± 2,3 h) e PN500 0h (32,4 ± 1,6 h). O menor tempo foi observado no grupo PN800 0h (21,9 h). O congelamento de células fetais bovinas de cultivo primário, realizado em palhetas de 0,25 mL, com 10% de DMSO, possibilita elevadas taxas de sobrevivência após o descongelamento. A PN modifica a curva de crescimento de células criopreservadas, sendo que as intensidades de 200 ou 500 mbar, aplicadas imediatamente antes do congelamento das células, possibilitam curvas de proliferação semelhantes às obtidas com células frescas.

Cell cryopreservation is an important tool in the preservation of endangered species. Fetal bovine primary culture-obtained cells were subjected to negative pressure (NP) 200, 500 or 800 mbar, just before (NP0h) or 3 hours before (NP3h) freezing into fine (0.25 mL) straws, using 10% DMSO as cryoprotectant. Fresh and frozen fibroblasts non submitted to NP were used as controls. We evaluated cell viability after freezing, cell proliferation curve, and population doubling time (PDT) every 24 hours during 8 days. Data were submitted to Tukey or Chi square test (P≤ 0.05). The average survival of control group (89.8%) and NP500-0h (88.1%) was higher than other groups; the time of PDT was similar in the fresh (27.5 ± 0.35 h), frozen control (30.1 ± 2.3 h) and NP500-0h groups (32.4 ± 1.6 h). The lowest time was observed in the NP800-0h (21.9 h) group. Freezing of bovine fibroblasts into 0.25 mL straws with 10% DMSO enables high survival rates after thawing. The NP modifies the growth curve of cryopreserved cells and the intensities of 200 or 500 mbar, applied just before freezing the cells, allow proliferation curves similar to those obtained with fresh cells.

Células fetais bovinas de cultivo primário submetidas a diferentes pressões negativas antes do congelamento em palhetas / Fetal bovine primary culture cells submitted to different negative pressures before straw freezing

O congelamento de células é uma importante ferramenta na preservação de espécies ameaçadas de extinção. Células fetais de cultivo primário obtidas de um bovino clone foram submetidas à pressão negativa (PN) de 200, 500 ou 800 mbar, imediatamente (PN0h) ou três horas antes (PN3h) do congelamento em palhetas finas, com 10% de DMSO como crioprotetor. Células frescas e congeladas sem submissão à PN foram utilizadas como controles. Avaliou-se a viabilidade pós-descongelamento, a curva de proliferação celular, assim como o tempo de duplicação da população (PDT) celular, a cada 24 horas, durante oito dias. Os dados obtidos foram submetidos ao teste de Tukey ou Qui quadrado (P≤0,05). A sobrevivência média dos grupos controle (89,8%) e PN500 0h (88,1%) foi superior aos outros grupos; o tempo de PDT foi semelhante nos grupos fresco (27,5 ± 0,35 h), controle congelado (30,1 ± 2,3 h) e PN500 0h (32,4 ± 1,6 h). O menor tempo foi observado no grupo PN800 0h (21,9 h). O congelamento de células fetais bovinas de cultivo primário, realizado em palhetas de 0,25 mL, com 10% de DMSO, possibilita elevadas taxas de sobrevivência após o descongelamento. A PN modifica a curva de crescimento de células criopreservadas, sendo que as intensidades de 200 ou 500 mbar, aplicadas imediatamente antes do congelamento das células, possibilitam curvas de proliferação semelhantes às obtidas com células frescas.(AU)

Cell cryopreservation is an important tool in the preservation of endangered species. Fetal bovine primary culture-obtained cells were subjected to negative pressure (NP) 200, 500 or 800 mbar, just before (NP0h) or 3 hours before (NP3h) freezing into fine (0.25 mL) straws, using 10% DMSO as cryoprotectant. Fresh and frozen fibroblasts non submitted to NP were used as controls. We evaluated cell viability after freezing, cell proliferation curve, and population doubling time (PDT) every 24 hours during 8 days. Data were submitted to Tukey or Chi square test (P≤ 0.05). The average survival of control group (89.8%) and NP500-0h (88.1%) was higher than other groups; the time of PDT was similar in the fresh (27.5 ± 0.35 h), frozen control (30.1 ± 2.3 h) and NP500-0h groups (32.4 ± 1.6 h). The lowest time was observed in the NP800-0h (21.9 h) group. Freezing of bovine fibroblasts into 0.25 mL straws with 10% DMSO enables high survival rates after thawing. The NP modifies the growth curve of cryopreserved cells and the intensities of 200 or 500 mbar, applied just before freezing the cells, allow proliferation curves similar to those obtained with fresh cells.(AU)

Intracytoplasmic sperm injection after vitrifcation of immature oocytes in follicular fluid increases bovine embryo production

Background: Despite the low efficiency caused by its harmful effects, vitrification is the technique of choice for oocyte cryopeservation, especially at the germinal vesicle (GV) stage. This enables the banking of female gametes without linkage to the male genotype. Follicular fluid (FF), in vivo, is known to provide an adequate environment to the immature oocyte. The intra-cytoplasmic sperm injection (ICSI), by the other hand, can be used to bypass any sperm penetration disorder, including the ones caused by cryopreservation. This study aimed to evaluate oocyte vitrification in FF based solution, and to asses ICSI efficiency in the fertilization of vitrified/warmed bovine GV oocytes. Material, Methods & Results: Follicles of 2-8 mm in diameter were aspirated from bovine ovaries obtained from a slaughterhouse, selected and maintained into FF from aspiration, until their allocation in the experimental groups. The FF used to prepare the vitrification solution was centrifuged, heat inactivated, filtered through a 0.22 mm pore and stored at -20°C. Oocyte vitrification was done into one of these three solutions: The standard solution TCM-Hepes (TH-Vitri) was compared to a totally FF based solution (FF-Vitri), and to a 50:50 (v/v) mix of both solutions (TH:FF-Vitri). Oocytes were submitted to in vitroembryo production in order to assess embryo production efficiency. A second set of experiments using the FF-Vitri solution compared IVF versus ICSI. With basis on cleaved structures, the morula + blastocyst rate obtained in the Fresh Control (43.9%) was similar to FF-Vitri (31.1%). Conversely, the TH-Vitri (15.7%) and the TH:FF-Vitri (20.4%) rates were significantly lower than the Fresh Control. ICSI showed a positive effect in comparison with IVF. The embryo development rate of Vitri-IVF (18.8%) was the lowest, whereas Vitri-ICSI (37.3%) was similar to the Fresh-IVF (43.9%), but lower than the Fresh-ICSI (57.8%).[...](AU)

Intracytoplasmic sperm injection after vitrifcation of immature oocytes in follicular fluid increases bovine embryo production

Background: Despite the low efficiency caused by its harmful effects, vitrification is the technique of choice for oocyte cryopeservation, especially at the germinal vesicle (GV) stage. This enables the banking of female gametes without linkage to the male genotype. Follicular fluid (FF), in vivo, is known to provide an adequate environment to the immature oocyte. The intra-cytoplasmic sperm injection (ICSI), by the other hand, can be used to bypass any sperm penetration disorder, including the ones caused by cryopreservation. This study aimed to evaluate oocyte vitrification in FF based solution, and to asses ICSI efficiency in the fertilization of vitrified/warmed bovine GV oocytes. Material, Methods & Results: Follicles of 2-8 mm in diameter were aspirated from bovine ovaries obtained from a slaughterhouse, selected and maintained into FF from aspiration, until their allocation in the experimental groups. The FF used to prepare the vitrification solution was centrifuged, heat inactivated, filtered through a 0.22 mm pore and stored at -20°C. Oocyte vitrification was done into one of these three solutions: The standard solution TCM-Hepes (TH-Vitri) was compared to a totally FF based solution (FF-Vitri), and to a 50:50 (v/v) mix of both solutions (TH:FF-Vitri). Oocytes were submitted to in vitroembryo production in order to assess embryo production efficiency. A second set of experiments using the FF-Vitri solution compared IVF versus ICSI. With basis on cleaved structures, the morula + blastocyst rate obtained in the Fresh Control (43.9%) was similar to FF-Vitri (31.1%). Conversely, the TH-Vitri (15.7%) and the TH:FF-Vitri (20.4%) rates were significantly lower than the Fresh Control. ICSI showed a positive effect in comparison with IVF. The embryo development rate of Vitri-IVF (18.8%) was the lowest, whereas Vitri-ICSI (37.3%) was similar to the Fresh-IVF (43.9%), but lower than the Fresh-ICSI (57.8%).[...]

Intracytoplasmic Sperm Injection after Vitrification of Immature Oocytes in Follicular Fluid Increases Bovine Embryo Production

Background: Despite the low efficiency caused by its harmful effects, vitrification is the technique of choice for oocyte cryopeservation, especially at the germinal vesicle (GV) stage. This enables the banking of female gametes without linkage to the male genotype. Follicular fluid (FF), in vivo, is known to provide an adequate environment to the immature oocyte. The intra-cytoplasmic sperm injection (ICSI), by the other hand, can be used to bypass any sperm penetration disorder, including the ones caused by cryopreservation. This study aimed to evaluate oocyte vitrification in FF based solution, and to asses ICSI efficiency in the fertilization of vitrified/warmed bovine GV oocytes.Material, Methods & Results: Follicles of 2-8 mm in diameter were aspirated from bovine ovaries obtained from a slaughterhouse, selected and maintained into FF from aspiration, until their allocation in the experimental groups. The FF used to prepare the vitrification solution was centrifuged, heat inactivated, filtered through a 0.22 mm pore and stored at -20C. Oocyte vitrification was done into one of these three solutions: The standard solution TCM-Hepes (TH-Vitri) was compared to a totally FF based solution (FF-Vitri), and to a 50:50 (v/v) mix of both solutions (TH:FF-Vitri). Oocytes were submitted to in vitro embryo production in order to assess embryo production efficiency. A second set

Intracytoplasmic Sperm Injection after Vitrification of Immature Oocytes in Follicular Fluid Increases Bovine Embryo Production

Background: Despite the low efficiency caused by its harmful effects, vitrification is the technique of choice for oocyte cryopeservation, especially at the germinal vesicle (GV) stage. This enables the banking of female gametes without linkage to the male genotype. Follicular fluid (FF), in vivo, is known to provide an adequate environment to the immature oocyte. The intra-cytoplasmic sperm injection (ICSI), by the other hand, can be used to bypass any sperm penetration disorder, including the ones caused by cryopreservation. This study aimed to evaluate oocyte vitrification in FF based solution, and to asses ICSI efficiency in the fertilization of vitrified/warmed bovine GV oocytes.Material, Methods & Results: Follicles of 2-8 mm in diameter were aspirated from bovine ovaries obtained from a slaughterhouse, selected and maintained into FF from aspiration, until their allocation in the experimental groups. The FF used to prepare the vitrification solution was centrifuged, heat inactivated, filtered through a 0.22 mm pore and stored at -20C. Oocyte vitrification was done into one of these three solutions: The standard solution TCM-Hepes (TH-Vitri) was compared to a totally FF based solution (FF-Vitri), and to a 50:50 (v/v) mix of both solutions (TH:FF-Vitri). Oocytes were submitted to in vitro embryo production in order to assess embryo production efficiency. A second set

Intracytoplasmic Sperm Injection after Vitrification of Immature Oocytes in Follicular Fluid Increases Bovine Embryo Production

Background: Despite the low efficiency caused by its harmful effects, vitrification is the technique of choice for oocyte cryopeservation, especially at the germinal vesicle (GV) stage. This enables the banking of female gametes without linkage to the male genotype. Follicular fluid (FF), in vivo, is known to provide an adequate environment to the immature oocyte. The intra-cytoplasmic sperm injection (ICSI), by the other hand, can be used to bypass any sperm penetration disorder, including the ones caused by cryopreservation. This study aimed to evaluate oocyte vitrification in FF based solution, and to asses ICSI efficiency in the fertilization of vitrified/warmed bovine GV oocytes.Material, Methods & Results: Follicles of 2-8 mm in diameter were aspirated from bovine ovaries obtained from a slaughterhouse, selected and maintained into FF from aspiration, until their allocation in the experimental groups. The FF used to prepare the vitrification solution was centrifuged, heat inactivated, filtered through a 0.22 mm pore and stored at -20C. Oocyte vitrification was done into one of these three solutions: The standard solution TCM-Hepes (TH-Vitri) was compared to a totally FF based solution (FF-Vitri), and to a 50:50 (v/v) mix of both solutions (TH:FF-Vitri). Oocytes were submitted to in vitro embryo production in order to assess embryo production efficiency. A second set

Intracytoplasmic Sperm Injection after Vitrification of Immature Oocytes in Follicular Fluid Increases Bovine Embryo Production

Background: Despite the low efficiency caused by its harmful effects, vitrification is the technique of choice for oocyte cryopeservation, especially at the germinal vesicle (GV) stage. This enables the banking of female gametes without linkage to the male genotype. Follicular fluid (FF), in vivo, is known to provide an adequate environment to the immature oocyte. The intra-cytoplasmic sperm injection (ICSI), by the other hand, can be used to bypass any sperm penetration disorder, including the ones caused by cryopreservation. This study aimed to evaluate oocyte vitrification in FF based solution, and to asses ICSI efficiency in the fertilization of vitrified/warmed bovine GV oocytes.Material, Methods & Results: Follicles of 2-8 mm in diameter were aspirated from bovine ovaries obtained from a slaughterhouse, selected and maintained into FF from aspiration, until their allocation in the experimental groups. The FF used to prepare the vitrification solution was centrifuged, heat inactivated, filtered through a 0.22 mm pore and stored at -20C. Oocyte vitrification was done into one of these three solutions: The standard solution TCM-Hepes (TH-Vitri) was compared to a totally FF based solution (FF-Vitri), and to a 50:50 (v/v) mix of both solutions (TH:FF-Vitri). Oocytes were submitted to in vitro embryo production in order to assess embryo production efficiency. A second set

Intracytoplasmic Sperm Injection after Vitrification of Immature Oocytes in Follicular Fluid Increases Bovine Embryo Production

Background: Despite the low efficiency caused by its harmful effects, vitrification is the technique of choice for oocyte cryopeservation, especially at the germinal vesicle (GV) stage. This enables the banking of female gametes without linkage to the male genotype. Follicular fluid (FF), in vivo, is known to provide an adequate environment to the immature oocyte. The intra-cytoplasmic sperm injection (ICSI), by the other hand, can be used to bypass any sperm penetration disorder, including the ones caused by cryopreservation. This study aimed to evaluate oocyte vitrification in FF based solution, and to asses ICSI efficiency in the fertilization of vitrified/warmed bovine GV oocytes.Material, Methods & Results: Follicles of 2-8 mm in diameter were aspirated from bovine ovaries obtained from a slaughterhouse, selected and maintained into FF from aspiration, until their allocation in the experimental groups. The FF used to prepare the vitrification solution was centrifuged, heat inactivated, filtered through a 0.22 mm pore and stored at -20C. Oocyte vitrification was done into one of these three solutions: The standard solution TCM-Hepes (TH-Vitri) was compared to a totally FF based solution (FF-Vitri), and to a 50:50 (v/v) mix of both solutions (TH:FF-Vitri). Oocytes were submitted to in vitro embryo production in order to assess embryo production efficiency. A second set

Intracytoplasmic Sperm Injection after Vitrification of Immature Oocytes in Follicular Fluid Increases Bovine Embryo Production

Background: Despite the low efficiency caused by its harmful effects, vitrification is the technique of choice for oocyte cryopeservation, especially at the germinal vesicle (GV) stage. This enables the banking of female gametes without linkage to the male genotype. Follicular fluid (FF), in vivo, is known to provide an adequate environment to the immature oocyte. The intra-cytoplasmic sperm injection (ICSI), by the other hand, can be used to bypass any sperm penetration disorder, including the ones caused by cryopreservation. This study aimed to evaluate oocyte vitrification in FF based solution, and to asses ICSI efficiency in the fertilization of vitrified/warmed bovine GV oocytes.Material, Methods & Results: Follicles of 2-8 mm in diameter were aspirated from bovine ovaries obtained from a slaughterhouse, selected and maintained into FF from aspiration, until their allocation in the experimental groups. The FF used to prepare the vitrification solution was centrifuged, heat inactivated, filtered through a 0.22 mm pore and stored at -20C. Oocyte vitrification was done into one of these three solutions: The standard solution TCM-Hepes (TH-Vitri) was compared to a totally FF based solution (FF-Vitri), and to a 50:50 (v/v) mix of both solutions (TH:FF-Vitri). Oocytes were submitted to in vitro embryo production in order to assess embryo production efficiency. A second set

Pre-incubation of porcine semen reduces the incidence of polyspermy on embryos derived from low quality oocytes / Pré-incubação dos espermatozoides suínos diminui polispermia e aumenta a produção embrionária em oócitos de baixa qualidade

The main cause of low efficiency of in vitro produced porcine embryos is the high polyspermic penetration rates at fertilization, which is aggravated in low quality oocytes. Experiment 1 evaluated the embryo development in high and low quality oocytes. Experiment 2 evaluated the embryo development and quality of low quality oocytes fertilized with sperm pre-incubated during 0h (control), 0.5h, 1h and 1.5h. Experiment 3 investigated fertilization and monospermic rates of the same groups of Experiment 2. Experiment 4 evaluated embryo development, cell density, fertilization and monospermic rates of high quality oocytes using semen pre incubated during the best time observed in the previous experiments. Cleavage and blastocyst rates were analyzed by chi-square test, and remaining data by ANOVA and Tukey test (P0.05). The cleavage (74.8 vs 51.7%) and blastocyst (33.7 vs 9.8%) rates were greater in oocytes of high versus low quality, with no differences in cell density. Fertilization rates (65.6 to 79.5%) were not influenced by pre-incubation time. However, semen pre-incubation during 1.5h increased monospermic penetration (53.3%) and cleavage rates (92.5%) in low quality oocytes. Blastocyst rate was improved with 1.5h of semen pre incubation; however they were still lower than that observed with high quality control oocytes. Ultimately, pre-incubation did not influence fertilization, monospermic penetration, embryo development rates, nor cell density in oocytes of high quality. Low-quality porcine oocytes resulted in better rates of embryo development if in vitro fertilized with sperm pre-incubated for 1.5 hour.(AU)

A principal causa da baixa eficiência na PIV de embriões suínos é a elevada taxa de polispermia, que é exacerbada em oócitos de baixa qualidade. O experimento 1 avaliou o desenvolvimento embrionário de oócitos de baixa e alta qualidade. O experimento 2 avaliou a qualidade e o desenvolvimento embrionário de oócitos de baixa qualidade fecundados com sêmen pré-incubado por 0h (controle), 0,5h, 1h e 1,5h. O experimento 3 investigou a fecundação e as taxas de monospermia dos mesmos grupos do experimento 2. O experimento 4 avaliou o desenvolvimento embrionário, a densidade celular, a fecundação e as taxas de monospermia de oócitos de alta qualidade, fecundados com sêmen pre-incubado com o melhor tempo observado nos experimentos anteriores. As taxas de clivagem e de blastocistos foram submetidas ao teste de Qui-quadrado e os demais dados submetidos à ANOVA e teste de Tukey (P0,05). As taxas de clivagem (74,8 vs 51,7%) e de blastocistos (33,7 vs 9,8%) foram superiores nos oócitos de alta qualidade, comparados aos de baixa qualidade, não havendo diferenças na quantidade de células embrionárias. As taxas de fecundação (65,6 vs 79,5%) não foram influenciadas pelo tempo de pré-incubação. Todavia, a pré-incubação do sêmen por 1,5h aumentou a penetração monospérmica (53,3%) e a taxa de clivagem (92,5%), nos oócitos de baixa qualidade. As taxas de blastocisto aumentaram com sêmen pré-incubado por 1,5h, que foram ainda inferiores às obtidas dos oócitos de alta qualidade do grupo controle. Finalmente, a pré-incubação do sêmen não influencia na fecundação, na penetração monospérmica, no desenvolvimento embrionário, nem na quantidade de células embrionárias com oócitos de alta qualidade. Oócitos suínos de baixa qualidade produzem melhores taxas de desenvolvimento embrionário se fecundados in vitro com sêmen pré-incubado por 1,5 horas.(AU)

Pre-incubation of porcine semen reduces the incidence of polyspermy on embryos derived from low quality oocytes / Pré-incubação dos espermatozoides suínos diminui polispermia e aumenta a produção embrionária em oócitos de baixa qualidade

ABSTRACT: The main cause of low efficiency of in vitro produced porcine embryos is the high polyspermic penetration rates at fertilization, which is aggravated in low quality oocytes. Experiment 1 evaluated the embryo development in high and low quality oocytes. Experiment 2 evaluated the embryo development and quality of low quality oocytes fertilized with sperm pre-incubated during 0h (control), 0.5h, 1h and 1.5h. Experiment 3 investigated fertilization and monospermic rates of the same groups of Experiment 2. Experiment 4 evaluated embryo development, cell density, fertilization and monospermic rates of high quality oocytes using semen pre incubated during the best time observed in the previous experiments. Cleavage and blastocyst rates were analyzed by chi-square test, and remaining data by ANOVA and Tukey test (P≤0.05). The cleavage (74.8 vs 51.7%) and blastocyst (33.7 vs 9.8%) rates were greater in oocytes of high versus low quality, with no differences in cell density. Fertilization rates (65.6 to 79.5%) were not influenced by pre-incubation time. However, semen pre-incubation during 1.5h increased monospermic penetration (53.3%) and cleavage rates (92.5%) in low quality oocytes. Blastocyst rate was improved with 1.5h of semen pre incubation; however they were still lower than that observed with high quality control oocytes. Ultimately, pre-incubation did not influence fertilization, monospermic penetration, embryo development rates, nor cell density in oocytes of high quality. Low-quality porcine oocytes resulted in better rates of embryo development if in vitro fertilized with sperm pre-incubated for 1.5 hour.

RESUMO: A principal causa da baixa eficiência na PIV de embriões suínos é a elevada taxa de polispermia, que é exacerbada em oócitos de baixa qualidade. O experimento 1 avaliou o desenvolvimento embrionário de oócitos de baixa e alta qualidade. O experimento 2 avaliou a qualidade e o desenvolvimento embrionário de oócitos de baixa qualidade fecundados com sêmen pré-incubado por 0h (controle), 0,5h, 1h e 1,5h. O experimento 3 investigou a fecundação e as taxas de monospermia dos mesmos grupos do experimento 2. O experimento 4 avaliou o desenvolvimento embrionário, a densidade celular, a fecundação e as taxas de monospermia de oócitos de alta qualidade, fecundados com sêmen pre-incubado com o melhor tempo observado nos experimentos anteriores. As taxas de clivagem e de blastocistos foram submetidas ao teste de Qui-quadrado e os demais dados submetidos à ANOVA e teste de Tukey (P≤0,05). As taxas de clivagem (74,8 vs 51,7%) e de blastocistos (33,7 vs 9,8%) foram superiores nos oócitos de alta qualidade, comparados aos de baixa qualidade, não havendo diferenças na quantidade de células embrionárias. As taxas de fecundação (65,6 vs 79,5%) não foram influenciadas pelo tempo de pré-incubação. Todavia, a pré-incubação do sêmen por 1,5h aumentou a penetração monospérmica (53,3%) e a taxa de clivagem (92,5%), nos oócitos de baixa qualidade. As taxas de blastocisto aumentaram com sêmen pré-incubado por 1,5h, que foram ainda inferiores às obtidas dos oócitos de alta qualidade do grupo controle. Finalmente, a pré-incubação do sêmen não influencia na fecundação, na penetração monospérmica, no desenvolvimento embrionário, nem na quantidade de células embrionárias com oócitos de alta qualidade. Oócitos suínos de baixa qualidade produzem melhores taxas de desenvolvimento embrionário se fecundados in vitro com sêmen pré-incubado por 1,5 horas.

Effects of exposure to halothane, isoflurane, and sevoflurane on embryo viability and gestation in female mice / Efeitos da exposição ao halotano, isofluorano, e sevofluorano na viabilidade embrionária e gestação em fêmeas de camundongos

Although the negative effects of inhalation anaesthetics on fertility have been known for a while, the stages during the reproductive cycle at which these effects occur and the mechanisms of action are largely unknown. This study aimed to evaluate the effects of acute exposure of female mice to halothane, isoflurane, and sevoflurane prior to mating. BALB/c female mice (n=160) were allocated in groups of 20 to halothane (HG), isoflurane (IG), sevoflurane (SG), and oxygen/sham (SH) treatment groups and their respective control groups (CGs). The mice were exposed to 1 minimum alveolar concentration (MAC) of the corresponding anaesthetic or oxygen for 4 h/day over 5 consecutive days. Two days after exposure, females were mated with males (ratio 2:1 female/male) for five consecutive days. Every morning, females were checked for the presence of vaginal plugs. Half of the females that exhibited plugs were euthanised 72 h later for embryo evaluation. The remaining females were euthanised on the 14th day of pregnancy for foetal evaluation. A low number of morulae and total embryos (morulae + blastocysts) were observed in the HG (P 0.05). The number of implantations was lower in the HG (6.0) compared with the IG (11.8) and SG (12.4) (P 0.05). Exposure to halothane is not recommended for use in female mice prior to mating procedures because it leads to decreased embryo production...(AU)

Embora os efeitos negativos dos anestésicos inalatórios na fertilidade já foram descritos há algum tempo, os estágios durante o ciclo reprodutivo em que estes efeitos ocorrem bem como os mecanismos de ação ainda permanecem desconhecidos. Os objetivos deste estudo foram avaliar os efeitos da exposição aguda em fêmeas de camundongos ao halotano, isofluorano, e sevofluorano prévio ao acasalamento. Fêmeas de camundongos BALB/c (n=160) foram alocadas em grupos de 20 aos tratamentos halotano (HG), isofluorano (IG), sevofluorano (SG), oxigênio (SH), e seus respectivos grupos controle (CGs). As fêmeas de camundongos foram expostas a uma concentração alveolar mínima (CAM) do anestésico correspondente ou a oxigênio por 4 horas diárias durante 5 dias consecutivos. Após dois dias do fim da exposição às fêmeas foram acasaladas com os machos (proporção 2:1 fêmea/macho) durante 5 dias consecutivos. A cada manhã, as fêmeas foram avaliadas para a observação da presença de plug vaginal. Metade das fêmeas que exibiam plug foram submetidas à eutanásia após 72 horas para avaliação embrionária. As fêmeas restantes foram eutanasiadas no 14º dia de gestação para avaliação fetal. No HG foi observado um menor número de mórulas e embriões totais (mórulas + blastocistos) (P 0,05). O número de implantações foi menor no HG (6,0) comparado ao IG (11,8) e SG (12,4) (P 0,05). A exposição ao halotano não...(AU)