Your search keyword '"C.O. Hidalgo"' showing total 33 results

1. Use of the flavonoid taxifolin for sperm cryopreservation from the threatened Bermeya goat breed

Author

J.N. Caamaño, J. Santiago-Moreno, F. Martínez-Pastor, C. Tamargo, A. Salman, Á. Fernández, M.J. Merino, E. Lacalle, A. Toledano-Díaz, and C.O. Hidalgo

Subjects

Food Animals, Equine, Animal Science and Zoology, Small Animals

Published

2023

2. Sperm chromatin condensation as an in vivo fertility biomarker in bulls: a flow cytometry approach

Author

Yentel Mateo-Otero, Jordi Ribas-Maynou, Marc Llavanera, Sandra Recuero, Ariadna Delgado-Bermúdez, R. Muiño, Sergi Bonet, Marc Yeste, Carolina Tamargo, C.O. Hidalgo, and AEI

Subjects

Cattle -- Spermatozoa, ADN -- Dany, Condensation, media_common.quotation_subject, Veterinary medicine, Fertility, Biology, Biochemistry, Bull, SF1-1100, Cryopreservation, Espermatozoides -- Investigació, Male infertility, Andrology, Cromatina, chemistry.chemical_compound, Bestiar boví -- Espermatozoides, In vivo, SF600-1100, medicine, Flow cytometry, reproductive and urinary physiology, media_common, Sperm chromatin condensation, urogenital system, Research, Sire, Chromomycin A3, medicine.disease, Sperm, Chromatin, Animal culture, chemistry, DNA damage, Animal Science and Zoology, Spermatozoa -- Research, Food Science, Biotechnology

Abstract

Background Genetic selection in cattle has been directed to increase milk production. This, coupled to the fact that the vast majority of bovine artificial inseminations (AI) are performed using cryopreserved sperm, have led to a reduction of fertility rates over the years. Thus, seeking sensitive and specific sperm biomarkers able to predict fertility rates is of vital importance to improve cattle reproductive efficiency. In humans, sperm chromatin condensation evaluated through chromomycin A3 (CMA3) has recently been purported to be a powerful biomarker for sperm functional status and male infertility. The objectives of the present study were: a) to set up a flow cytometry method for simultaneously evaluating chromatin condensation and sperm viability, and b) to test whether this parameter could be used as a predictor of in vivo fertility in bulls. The study included pools of three independent cryopreserved ejaculates per bull from 25 Holstein males. Reproductive outcomes of each sire were determined by non-return rates, which were used to classify bulls into two groups (highly fertile and subfertile). Results Chromatin condensation status of bovine sperm was evaluated through the combination of CMA3 and Yo-Pro-1 staining and flow cytometry. Sperm quality parameters (morphology, viability, total and progressive motility) were also assessed. Pearson correlation coefficients and ROC curves were calculated to assess their capacity to predict in vivo fertility. Sperm morphology, viability and total motility presented an area under the ROC curve (AUC) of 0.54, 0.64 and 0.68, respectively (P > 0.05), and thus were not able to discriminate between fertile and subfertile individuals. Alternatively, while the percentage of progressively motile sperm showed a significant predictive value, with an AUC of 0.73 (P = 0.05), CMA3/Yo-Pro-1 staining even depicted superior results for the prediction of in vivo fertility in bulls. Specifically, the percentage of viable sperm with poor chromatin condensation showed better accuracy and precision to predict in vivo fertility, with an AUC of 0.78 (P = 0.02). Conclusions Chromatin condensation evaluated through CMA3/Yo-Pro-1 and flow cytometry is defined here as a more powerful tool than conventional sperm parameters to predict bull in vivo fertility, with a potential ability to maximising the efficiency of dairy breeding industry.

Published

2021

3. Supplementation of the BIOXcell extender with the antioxidants crocin, curcumin and GSH for freezing bull semen

Author

J. Néstor Caamaño, Felipe Martínez-Pastor, Carolina Tamargo, Ángel Fernández, María J. Merino, Amer Salman, Touba Nadri, Estela Fernández-Alegre, Carmen Fueyo, and C.O. Hidalgo

Subjects

Male, Curcumin, 040301 veterinary sciences, Semen, Antioxidants, Cryopreservation, law.invention, 0403 veterinary science, Crocin, Andrology, 03 medical and health sciences, chemistry.chemical_compound, Capacitation, law, Animals, 030304 developmental biology, 0303 health sciences, General Veterinary, Extender, 04 agricultural and veterinary sciences, Glutathione, Carotenoids, Semen cryopreservation, Culture Media, chemistry, Sperm Motility, Cattle, Semen Preservation

Abstract

Semen cryopreservation is routine in cattle, but the results of artificial insemination need improvement. A strategy to these aims is the supplementation of the freezing extender with novel antioxidants. This study aimed at testing the natural antioxidants curcumin and crocin as supplements to the commercial extender BIOXcell for freezing semen from 8 Holstein bulls. We tested curcumin at 0.05 and 0.1 mM (CU0.05, CU0.1) and crocin at 0.5 and 1.5 mM (CR0.5, CR1.5), with 0.5 mM reduced glutathione (GSH0.5) as reference, and a control (CTL, without supplementation). The samples were evaluated post-thawing and after 5 h at 38 °C by CASA for motility and flow cytometry for viability, apoptotic, capacitation, acrosomal status, cytoplasmic and mitochondrial reactive oxygen species (ROS) production, and chromatin status (SCSA). Control and GSH0.5 showed similar results, possibly because of the good protection from BIOXcell. CU0.05 and CU0.1 showed little effects but increased cytoplasmic ROS production and motility ALH. CR0.5 and CR1.5 decreased viability and increased apoptotic features significantly post-thawing and after the incubation, resulting in lower motility (significant after the incubation) but decreasing SCSA %HDS (loose chromatin). Whereas crocin at these concentrations seems incompatible with BIOXcell, maybe because of a prooxidant activity, curcumin use merits further research, considering the elevation of ROS with no significant negative effects.

Published

2021

4. Effect of oviductal fluid on bull sperm functionality and fertility under non-capacitating and capacitating incubation conditions

Author

Joaquín Gadea, Raquel Romar, Jordana S. Lopes, Niyazi Küçük, Cristina Soriano-Úbeda, and C.O. Hidalgo

Subjects

Male, endocrine system, animal structures, Acrosome reaction, Semen, Insemination, Andrology, 03 medical and health sciences, 0302 clinical medicine, Human fertilization, Food Animals, Capacitation, Animals, Small Animals, Acrosome, Fallopian Tubes, reproductive and urinary physiology, 030219 obstetrics & reproductive medicine, urogenital system, Equine, Chemistry, Acrosome Reaction, 0402 animal and dairy science, Embryo culture, 04 agricultural and veterinary sciences, Spermatozoa, 040201 dairy & animal science, Sperm, Fertility, Sperm Motility, Cattle, Female, Animal Science and Zoology, Sperm Capacitation

Abstract

This study investigated the effect of bovine oviductal fluid from late follicular (LF) and early luteal (EL) phases on bull sperm functionality under non-capacitating (NCAP) and capacitating (CAP) conditions. Frozen-thawed semen samples from five bulls were thawed and incubated (0, 1 or 2 h) in NCAP and CAP media supplemented with 1% bovine oviductal fluid (LF and EL groups) and in absence of fluid (C group). Motion parameters were assessed by CASA; sperm viability, acrosomal integrity and membrane lipid disorder parameters were evaluated by flow cytometry; and sperm DNA fragmentation was evaluated by the Comet assay. Finally, in vitro fertilization with sperm treated under CAP conditions was performed and further embryo culture results evaluated. In NCAP medium, addition of LF and EL fluid increased the total and progressive motility, and LF fluid improved the stability of sperm DNA. However, under CAP conditions addition of LF and EL fluid decreased some sperm motion parameters and some parameters of sperm DNA stability. Proportion of viable sperm cells with low lipid disorder was higher in NCAP than CAP medium and addition of LF fluid markedly increased the proportion of viable spermatozoa with high lipid disorder and acrosome alteration (spontaneous acrosome reaction). Under current conditions, incubation of bull sperm with oviductal fluid before insemination did not affect detrimentally the IVF results nor embryo development, being blastocyst rate similar between CAP-LF, CAP-EL and control groups. In conclusion, oviductal fluid positively influences sperm functionality and modulate in vitro capacitation.

Published

2020

5. Post-Thaw Sperm Quality and Functionality in the Autochthonous Pig Breed Gochu Asturcelta

Author

Amer Salman, María J. Merino, Carmen Fueyo, Tania Iglesias, Inmaculada Parrilla, Felipe Martínez-Pastor, Lorena Padilla, José Néstor Caamaño, C.O. Hidalgo, Carolina Tamargo, and Ángel Fernández

Subjects

pig, endocrine system, sperm quality, BOAR, Veterinary medicine, Semen, Biology, Article, 03 medical and health sciences, 0302 clinical medicine, Animal science, SF600-1100, Fragmentation (cell biology), Sperm quality, Incubation, 030219 obstetrics & reproductive medicine, General Veterinary, urogenital system, seasonality, 0402 animal and dairy science, 04 agricultural and veterinary sciences, 040201 dairy & animal science, Sperm, Semen cryopreservation, Breed, sperm cryopreservation, QL1-991, Animal Science and Zoology, autochthonous breeds, Zoology, hormones, hormone substitutes, and hormone antagonists

Abstract

Genetic resource banks (GRB) preserve the genetic material of endangered, valuable individuals or genetically relevant breeds. Semen cryopreservation is a crucial technique to reach these goals. Thus, we aimed to assess the sperm parameters of semen doses from the native pig breed Gochu Asturcelta stored at the GRB of Principado de Asturias (GRB-PA, Gijón, Spain), focusing on intrinsic and extrinsic (boar, season) factors. Two straws per boar (n = 18, 8–71 months of age) were thawed, pooled, and assessed after 30 and 150 min at 37 °C by CASA (computer-assisted sperm analysis system, motility and kinematic parameters) and flow cytometry (viability, acrosomal status, mitochondrial activity, apoptosis, reactive oxygen species, and chromatin status). The effects of age, incubation, and season on post-thawing quality were determined using linear mixed-effects models. Parameters were on the range for commercial boar breeds, with chromatin status (SCSA: fragmentation and immaturity) being excellent. Incubation decreased sperm quality and functionality. The boar age did not have a significant effect (p &gt, 0.05), but the between-boar variability was significant (p &lt, 0.001). The season significantly affected many parameters (motility, kinematics, viability, acrosomal status, mitochondrial activity), especially after 150 min of incubation. In general, samples collected in spring and summer showed higher quality post-thawing, the lowest in winter. In conclusion, the sperm doses from the Gochu Asturcelta breed stored at the GRB-PA showed excellent chromatin status and acceptable characteristics after thawing. Therefore, boar and seasonal variability in this autochthonous breed could be relevant for cryobank management.

Published

2021

6. A Shorter Equilibration Period Improves Post-Warming Outcomes after Vitrification and in Straw Dilution of In Vitro-Produced Bovine Embryos

Author

Meritxell Vendrell-Flotats, Joseba Esmoris, Sabino Azcarate, Xabier Mendibil, Iris Martínez-Rodero, Teresa Mogas, C.O. Hidalgo, Tania García-Martínez, Erika Alina Ordóñez-León, Marc Yeste, and Manel Lopez-Bejar

Subjects

total cell number, SOX2, cow, Apoptosis, cryopreservation, Cryopreservation, 0302 clinical medicine, Inner cell mass, Vitrification, Reproducció assistida, lcsh:QH301-705.5, TUNEL, Expanded blastocyst, 030219 obstetrics & reproductive medicine, Bestiar boví -- Embrions, apoptosis, Embryo, 04 agricultural and veterinary sciences, Straw, inner cell mass, Dilution, expanded blastocyst, embryonic structures, Trophectoderm, trophectoderm, General Agricultural and Biological Sciences, animal structures, Cattle -- Embryos, Biology, General Biochemistry, Genetics and Molecular Biology, Article, Andrology, 03 medical and health sciences, Regulació genètica, Genetic regulation, General Immunology and Microbiology, Hatching, Cow, 0402 animal and dairy science, Total cell number, Reproductive technology, Expressió gènica, 040201 dairy & animal science, In vitro, lcsh:Biology (General), gene expression, Gene expression

Abstract

This study was designed to the optimize vitrification and in-straw warming protocol of in vitro-produced bovine embryos by comparing two different equilibration periods, short equilibrium (SE: 3 min) and long equilibrium (LE: 12 min). Outcomes recorded in vitrified day seven (D7) and day eight (D8) expanded blastocysts were survival and hatching rates, cell counts, apoptosis rate, and gene expression. While survival rates at 3 and 24 h post-warming were reduced (p &lt, 0.05) after vitrification, the hatching rates of D7 embryos vitrified after SE were similar to the rates recorded in fresh non-vitrified blastocysts. The hatching rates of vitrified D8 blastocysts were lower (p &lt, 0.05) than of fresh controls regardless of treatment. Total cell count, and inner cell mass and trophectoderm cell counts were similar in hatched D7 blastocysts vitrified after SE and fresh blastocysts, while vitrified D8 blastocysts yielded lower values regardless of treatment. The apoptosis rate was significantly higher in both treatment groups compared to fresh controls, although rates were lower for SE than LE. No differences emerged in BAX, AQP3, CX43, and IFNτ gene expression between the treatments, whereas a significantly greater abundance of BCL2L1 and SOD1 transcripts was observed in blastocysts vitrified after SE. A shorter equilibration vitrification protocol was found to improve post-warming outcomes and time efficiency after in-straw warming/dilution.

Published

2021

7. Inhibiting diacylglycerol acyltransferase-1 reduces lipid biosynthesis in bovine blastocysts produced in vitro

Author

Cláudia Lima Verde Leal, Y. N. Cajas, N. Vásquez, Dimitrios Rizos, P. Beltrán-Breña, Karina Cañón-Beltrán, J. Giraldo-Giraldo, C.O. Hidalgo, Encina M González, and Alfonso Gutiérrez-Adán

Subjects

Fertilization in Vitro, Andrology, Embryo Culture Techniques, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Food Animals, Lipid droplet, Lipid biosynthesis, medicine, Animals, Blastocyst, Diacylglycerol O-Acyltransferase, Small Animals, Diacylglycerol kinase, Cryopreservation, 030219 obstetrics & reproductive medicine, Equine, Dimethyl sulfoxide, 0402 animal and dairy science, Embryo, 04 agricultural and veterinary sciences, 040201 dairy & animal science, Lipids, In vitro, medicine.anatomical_structure, chemistry, Oviduct, Animal Science and Zoology, Cattle

Abstract

Diacylglycerol acyltransferase-1 (DGAT1) is one of the DGAT enzymes that catalyzes the final step in the synthesis of triacylglycerol, which is a major component of the lipid droplets in embryos. Intracellular lipids accumulated in embryos produced in vitro have been associated with reduced cryotolerance and quality. The objective of the present study was to investigate the influence of DGAT1 inhibition on embryo development, quality, and post-vitrification survival, in addition to expression profiles of selected lipid metabolism-regulating and oxidative stress genes. Bovine cumulus-oocyte complexes were matured and fertilized in vitro and were cultured in synthetic oviduct fluid (SOF) supplemented with 5% fetal calf serum (FCS) alone (Control) or with 1, 5, 10 or 50 μM DGAT1 inhibitor (A922500®; D1, D5, D10, and D50, respectively) or 0.1% dimethyl sulfoxide (CDMSO: vehicle for DGAT1 inhibitor dilution) from 54 h post-insemination until Day 8 post insemination. No differences were found in blastocyst yield on days 7 and 8 in Control, CDMSO, D10, and D50 groups. Embryos cultured with 10 or 50 μM DGAT1 inhibitor had greater mitochondrial activity (P 0.01), and increased number of cells (P 0.05), while the cytoplasmic lipid content was reduced (P 0.01), the latter associated with altered expression profiles of selected genes regulating lipid metabolism or genes related with oxidative stress (transcript abundance increased for SLC2A1 and SLC2A5 and decreased for DGAT1 and GPX1). Importantly, the survival rate of blastocysts produced with 10 μM DGAT1 was higher than that of Control, CDMSO and D50 groups at 72 h after vitrification and warming (73.8 vs 57.1, 55.9 and 56.1%, respectively, P 0.001). In conclusion, inhibition of DGAT1 synthesis in bovine embryos produced in vitro abrogates the negative effect of FCS by decreasing their lipid content, increasing mitochondria activity and improving embryo cryotolerance, as well as favoring the expression of lipid metabolism regulating and oxidative stress-related transcripts.

Published

2020

8. Changes in the Cellular Distribution of Tyrosine Phosphorylation and Its Relationship with the Acrosomal Exocytosis and Plasma Membrane Integrity during In Vitro Capacitation of Frozen/Thawed Bull Spermatozoa

Author

Sara Ruiz-Díaz, Sergio Grande-Pérez, C.O. Hidalgo, Serafín Pérez-Cerezales, Sol Arce-López, and Carolina Tamargo

Subjects

0301 basic medicine, Male, Acrosome reaction, bull spermatozoa, environment and public health, lcsh:Chemistry, chemistry.chemical_compound, 0302 clinical medicine, Freezing, Phosphorylation, lcsh:QH301-705.5, Spectroscopy, Calcimycin, 030219 obstetrics & reproductive medicine, General Medicine, Spermatozoa, Computer Science Applications, Cell biology, Calcium Ionophores, Sperm Motility, Acrosome, Intracellular, animal structures, acrosome reaction, chemistry.chemical_element, Calcium, Catalysis, Exocytosis, Article, sperm capacitation, Inorganic Chemistry, 03 medical and health sciences, Capacitation, protein tyrosine phosphorylation, Centrifugation, Density Gradient, Animals, Physical and Theoretical Chemistry, Molecular Biology, urogenital system, Organic Chemistry, Cell Membrane, Tyrosine phosphorylation, Sperm, enzymes and coenzymes (carbohydrates), 030104 developmental biology, chemistry, lcsh:Biology (General), lcsh:QD1-999, membrane integrity, Tyrosine, Cattle

Abstract

During sperm capacitation, intracellular signaling leads to protein tyrosine phosphorylation (PTP) of multiple cellular structures. However, the connection of this molecular signaling to the physiology of capacitated spermatozoa is not completely understood. This is the case of the short lifespan of capacitated spermatozoa and their increased susceptibility to initiate acrosomal exocytosis (AE) during incubation. Herein, by employing frozen/thawed bull spermatozoa, we aimed to study the relationship between PTP with AE and with plasma membrane integrity (PMI) at the cellular level. For this, we employed double staining following immunofluorescence for PTP combined with fluorescence probes for the acrosome (PNA-FITC) and PMI (LIVE/DEAD Fixable Dead Cell Stain Kit). Our results revealed that the presence of PTP at sperm head was less abundant in the sperm fraction that triggered the AE after 3 h of incubation under capacitating conditions, or by its induction with calcium ionophore, compared to the unreacted fraction. Furthermore, PTP at the equatorial region of the head (PTP-EQ) was enriched in the fraction showing damaged membrane while induction of AE with calcium ionophore did not alter the PMI and its relation to PTP-EQ. These results suggest that spontaneous AE and induced AE trigger similar cellular events regarding PTP and the spermatozoa showing PTP-EQ are more prone to suffer plasma membrane damage.

Published

2020

9. Ability of the ISAS3Fun Method to Detect Sperm Acrosome Integrity and Its Potential to Discriminate between High and Low Field Fertility Bulls

Author

Carolina Tamargo, Pilar Santolaria, Jesús Yániz, M.A. Silvestre, Inmaculada Palacín, and C.O. Hidalgo

Subjects

capacitation, endocrine system, QH301-705.5, Sperm Head, animal diseases, media_common.quotation_subject, Acrosome reaction, Bos taurus, acrosome reaction, Semen, Fertility, Biology, Article, male fertility, General Biochemistry, Genetics and Molecular Biology, Andrology, fluids and secretions, Capacitation, Biology (General), Acrosome, reproductive and urinary physiology, Sperm motility, media_common, General Immunology and Microbiology, urogenital system, spermiogram, Sperm, General Agricultural and Biological Sciences

Abstract

The objective of the present study was to investigate whether fertility differences in bulls are reflected in variations of sperm quality when analysing only one ejaculate per male. Two experiments were performed. In the first experiment, frozen semen samples from 20 adult bulls were tested, 10 bulls had high field fertility and 10 bulls had low field fertility. Analyses of sperm motility, membrane integrity, and membrane–acrosome integrity with the ISAS3Fun method were performed. Sperm morphometry of the fluorescence sperm subpopulations obtained with the ISAS3Fun method was also analysed. Significant differences between high- and low-fertility groups were only found with the ISAS3Fun technique, specifically in sperm acrosome integrity, the proportion of spermatozoa with an intact acrosome and damaged membrane, and in sperm head width of spermatozoa with intact structures. Discriminant analyses allowed us to correctly classify 90% of sperm samples in their fertility group using sperm quality parameters. Given that only the results obtained with the ISAS3Fun technique were related to bull fertility, we performed a second experiment aimed to validate the efficacy of this technique to detect the acrosomal integrity of bull spermatozoa, comparing them with the conventional FITC-PNA/propidium iodide (PNA/PI) combination under capacitating conditions. The results indicated that the ISAS3Fun combination provided an accurate assessment of both viability and acrosomal integrity for ejaculated spermatozoa, while the PNA/PI combination underestimated the extension of acrosomal damage due to false negatives. It was concluded that the simultaneous assessment of sperm plasma membranes and acrosome integrity with the ISAS3Fun method is precise and seems to have a greater potential to discriminate between high- and low-fertility bulls than more conventional in vitro sperm quality tests.

Published

2021

10. A comparative study of the sperm nuclear morphometry in cattle, goat, sheep, and pigs using a new computer-assisted method (CASMA-F)

Author

Jesús Yániz, Pilar Santolaria, F. Arrebola, M.A. Silvestre, Inmaculada Palacín, C.O. Hidalgo, and S. Vicente-Fiel

Subjects

Male, endocrine system, BOAR, Swine, Sperm Head, Semen, Biology, Andrology, Species Specificity, Food Animals, Image Processing, Computer-Assisted, Animals, Air drying, Small Animals, Fluorescent Dyes, Cell Nucleus, Sheep, urogenital system, Equine, Goats, Anatomy, Spermatozoa, Sperm, Open software, Microscopy, Fluorescence, Benzimidazoles, Cattle, Animal Science and Zoology

Abstract

This study was designed to compare the sperm nuclear morphometry of four species of domestic artiodactyls (cattle, sheep, goats, and pigs), using the newly developed automatic computer-assisted sperm morphometry analysis-F. The study was divided into two experiments. In the first experiment, samples from 20 males from each species were collected, diluted, and divided into four sample aliquots. The first was labeled directly with Hoechst 33342, and the others were processed as smears. Between smears, one group was directly labeled with Hoechst after air drying, and the other was fixed either with glutaraldehyde (GLUT), or with methanol, and afterward labeled with Hoechst. Digital images of the fluorescence-labeled sperm were recorded with a digital camera, and at least 200 sperm cells per sample were processed using the Image J analysis open software. Air-drying significantly reduced nuclear sperm dimensions in ruminant species, whereas no effect was observed in pigs. For most of the primary morphometric parameters, the relationship between the four species for the sperm nuclear dimensions can be described as follows: bull > ram ≥ boar > goat. However, ram sperm nuclei had greater width than those of the other species studied. For the secondary morphometric parameters, ram sperm nuclei were clearly less elliptical and elongated and showed greater regularity than in the other studied species. In the second experiment, ejaculates from 10 males per species were used to compare the sperm head morphometric results obtained with the computer-assisted sperm morphometry analysis-F system (using the GLUT treatment as reference) to a more conventional CASMA method (semen smears stained with Harris's hematoxylin and processed with the Integrated Sperm Analysis System [ISAS] commercial software [Proiser R&D SL, Bunol, Spain]). Spermatozoa displayed a bigger size when processed with Harris's hematoxylin than with the GLUT method in all primary sperm head morphometric parameters for the four species studied. A significant correlation was observed between the two methods used in this experiment for all morphometric size parameters in the four species studied. It was concluded that drying and fixation has little effect on sperm nuclear morphometry, with differences between species, and that there are significant variations in size of the sperm nucleus and in the hydrodynamic properties between the four species studied.

Published

2013

11. Ultrastructure and Development of Vitrified/Warmed Bovine Oocytes Matured with 9-cis Retinoic Acid

Author

Enrique J. Gómez, C.O. Hidalgo, P. Duque, N. Facal, Aida Rodríguez, Carolina Tamargo, José Néstor Caamaño, M. Carbajo, Isaac Antolín, Cristina Alonso, L. Fernandez, and Carmen Díez

Subjects

Cis-Retinoic Acid, medicine.anatomical_structure, Immunology, Biomedical Engineering, Ultrastructure, medicine, Vitrification, Cell Biology, Biology, Oocyte, General Biochemistry, Genetics and Molecular Biology, Biotechnology, Cell biology

Abstract

In this work we analyze the effects of vitrification on the ultrastructure and developmental ability of bovine oocytes matured in the presence of 9-cis-retinoic acid (RA). Bovine cumulus oocyte com...

Published

2006

12. Intrauterine Neospora caninum inoculation of heifers

Author

G. Aduriz, Raquel Atxaerandio, Ignacio Ferre, Luis Miguel Ortega-Mora, A. Martínez, Koldo Osoro, C.O. Hidalgo, E. Serrano, and A. Mateos-Sanz

Subjects

Embryo, Nonmammalian, animal structures, animal diseases, medicine.medical_treatment, Cattle Diseases, Semen, Andrology, Interferon-gamma, Random Allocation, Neospora, parasitic diseases, medicine, Animals, Seroconversion, Insemination, Artificial, General Veterinary, biology, Coccidiosis, Artificial insemination, Brain, Embryo, General Medicine, DNA, Protozoan, Embryo, Mammalian, biology.organism_classification, Infectious Disease Transmission, Vertical, Neospora caninum, Organ Specificity, In utero, Immunology, biology.protein, Cattle, Female, Parasitology, Antibody

Abstract

Here, we studied the potential of Neospora caninum tachyzoites to infect heifers when administered in utero by artificial insemination via contaminated semen. Eighteen primiparous cyclic heifers were hormonally synchronized and artificially inseminated. Nine of them, which were inseminated with semen containing 10 7 live N. caninum NC-1 isolate-tachyzoites, reacted with seroconversion and a specific IFN-γ response. Moreover, N. caninum DNA was demonstrated by a nested-PCR in the blood of all nine heifers and in brain, lungs, liver and uterine horn of several of them. In contrast, nine heifers inseminated with tachyzoite-free semen developed no antibody or IFN-γ responses, and no parasite DNA was detected in blood or organs. At necropsy, viable embryos were detected in one and six of the infected and non-infected heifers, respectively. No specific Neospora DNA was detected in any of the embryos. This study provides evidence that intrauterine inoculation via contaminated semen cause N. caninum infection in cattle.

Published

2006

13. Pregnancy rates and metabolic profiles in cattle treated with propylene glycol prior to embryo transfer

Author

Félix Goyache, P. Duque, Itziar Fernández, N. Facal, L. Fernandez, C.O. Hidalgo, Carmen Díez, Enrique J. Gómez, and Lupicinio Prieto

Subjects

Blood Glucose, medicine.medical_specialty, Hot Temperature, Pregnancy Rate, medicine.medical_treatment, Ice calving, Biology, chemistry.chemical_compound, Estrus, Food Animals, Pregnancy, Internal medicine, medicine, Animals, Insulin, Urea, Insulin-Like Growth Factor I, Small Animals, Progesterone, Triglycerides, Cryopreservation, Estrous cycle, Triglyceride, Equine, Pregnancy Outcome, Embryo Transfer, Embryo, Mammalian, medicine.disease, Propylene Glycol, Embryo transfer, Endocrinology, medicine.anatomical_structure, chemistry, Cattle, Female, Animal Science and Zoology, Corpus luteum

Abstract

The objective of this study was to determine the effect of a sustained propylene glycol administration to recipients of frozen/thawed in vivo derived bovine embryos. Heifers were treated with oral propylene glycol for the last 20 days before embryo transfer (n = 142), and untreated as controls (n = 133). Progesterone, insulin, insulin-like growth factor-I, glucose, urea and triglyceride were analysed in blood on Day 0 and Day 7 of the estrous cycle corresponding to embryo transfer. The heifers were selected as recipients when showing progesterone levels2.0 ng/ml (Day 0) and2.5 ng/ml (Day 7), according to corpus luteum quality on Day 7 by technicians unaware of animals treated. Within treated animals, significantly more recipients were selected, and increased progesterone, corpus luteum quality, pregnancy and calving rates were recorded. Day 7 progesterone concentrations were higher in heifers treated and transferred. Propylene glycol increased insulin and insulin-like-growth factor-I, but glucose, urea and triglyceride did not vary. Furthermore, insulin-like-growth factor-I, glucose and triglyceride increased at estrous time, but urea decreased and insulin remained unaltered. Together with the sustained gain in pregnancy rates throughout the experiment (2 years), other evidences suggested that the observed effects did not rely on nutritional deficiency. Thus, propylene glycol improved pregnancy rates after embryo-transfer, and progesterone, insulin and insulin-like-growth factor-I are probably involved in this effect.

Published

2004

14. 9-cis-retinoic acid during in vitro maturation improves development of the bovine oocyte and increases midkine but not IGF-I expression in cumulus-granulosa cells

Author

Isabel Álvarez, Gustavo Ferrer Carneiro, Luis-José Royo, P. Duque, Pedro Lorenzo, C.O. Hidalgo, Carmen Díez, Enrique J. Gómez, N. Facal, and Félix Goyache

Subjects

Midkine, Retinoic acid, Embryo, Cell Biology, Biology, Oocyte, Molecular biology, Cryopreservation, In vitro, In vitro maturation, Andrology, chemistry.chemical_compound, medicine.anatomical_structure, chemistry, Gene expression, Genetics, medicine, biology.protein, Developmental Biology

Abstract

The isomer 9-cis of retinoic acid (9-cis-RA) exerts a beneficial effect on bovine in vitro development when added to in vitro maturation (IVM) culture. In the present work, 9-cis-RA 5 nM was found to be stimulatory as opposed to 500 nM (toxic). Cumulus-oocyte complexes (COCs) were treated with the found physiological dose 9-cis-RA 5 nM, and the next determinations performed: (1) relative expression of midkine (MK) and IGF-I, by reverse transcriptase- polymerase chain reaction (RT-PCR), in cumulus- granulosa cells detached from oocytes; (2) cytoplasmic granular migration, by labeling of oocytes with fluoro- scein isothiocyanate lectins; and (3) in vitro survival of blastocysts after vitrification and warming. Gene expression of MK was enhanced by 9-cis-RA, but not by 1% ethanol (vehicle). However, we did not detect IGF-I expression, both in dependence on or in the absenceof9-cis-RAactingoncumulus-granulosacells. The ability of vitrified blastocysts to survive in vitro was not improved by 9-cis-RA. Nevertheless, since only blastocysts obtained from oocytes matured with serum survived, more factors should be considered when evaluating cryopreservation survival. The complete granular migration observed in oocytes matured with 9-cis-RA anticipates the gain in developmental com- petence of the oocyte, being MK probably involved in this beneficial effect. Mol. Reprod. Dev. 66: 247- 255, 2003. 2003 Wiley-Liss, Inc.

Published

2003

15. Use of two replacements of serum during bovine embryo culture in vitro

Author

P. Duque, C.O. Hidalgo, Carmen Díez, E. Díaz, Enrique J. Gómez, and N. Facal

Subjects

Zygote, Cell Count, Fertilization in Vitro, Biology, Morula, Andrology, Embryonic and Fetal Development, Food Animals, Culture Techniques, medicine, Animals, Inner cell mass, Bovine embryo, Blastocyst, Small Animals, Equine, Embryogenesis, Embryo culture, Embryo, Embryo Transfer, In vitro, Culture Media, medicine.anatomical_structure, embryonic structures, Immunology, Cattle, Female, Animal Science and Zoology

Abstract

This study evaluated the effect of two commercial serum replacements (Ultroser G and CPSR-3 on in vitro bovine embryo culture. In Experiment 1, zygotes were cultured in SOF+Ultroser G (2, 4 and 6%), SOF+CPSR-3 (2, 4 and 6%), and SOF+5% FCS (control). Blastocyst rates obtained after culturing with Ultroser G were lower than those with FCS. However, blastocyst rates for CPSR-3 were similar to those for serum. In addition, embryos produced in SOF+CPSR-3 had the same proportion inner cell mass number and total cell number as embryos cultured with FCS. In Experiment 2, a combination of serum replacements during different periods showed that treatment before the five-to eight-cell stages had no effect on further embryo development. However, treatments up to the morula stage affected blastocyst formation. The concentration of supplement and the timing of its inclusion in culture markedly affected embryo development. The serum replacement CPSR-3 can supplement embryo culture with blastocyst rates and quality similar to those for serum.

Published

2003

16. Effects of acetoacetate and d-β-hydroxybutyrate on bovine in vitro embryo development in serum-free medium

Author

C.O. Hidalgo, E. Díaz, Carmen Díez, N. Facal, Isaac Antolín, Enrique J. Gómez, and P. Duque

Subjects

animal structures, Fertilization in Vitro, Biology, Morula, Culture Media, Serum-Free, Acetoacetates, Embryonic and Fetal Development, Food Animals, Culture Techniques, medicine, Animals, 3-Hydroxybutyric Acid, Blastocyst, Small Animals, Equine, Embryogenesis, Embryo, Embryo Transfer, In vitro, Embryo transfer, medicine.anatomical_structure, Biochemistry, embryonic structures, Ketone bodies, Oviduct, Cattle, Female, Animal Science and Zoology

Abstract

It is known that the ketone bodies acetoacetate and D-beta-hydroxybutyrate can be metabolized by the early bovine embryo for in vitro development. In the present work, we report experiments leading to the culture of bovine embryos in the absence of serum. In vitro-produced bovine zygotes were cultured in modified synthetic oviduct fluid medium supplemented with acetoacetate derivatives, acetoacetate and D-beta-hydroxybutyrate. Acetoacetate and its derivatives prevented blastocysts from forming in the absence of serum during the whole culture period. However, from Days 6 to 8 of culture in the absence of serum, acetoacetate did not affect development as compared to controls containing lactate and pyruvate or no substrate. Interestingly, D-beta-hydroxybutyrate stimulated blastocyst and expansion development, and allowed lipid mobilization. In feeder cells coculture, embryos produced with D-beta-hydroxybutyrate showed improved hatching. Embryos cultured in D-beta-hydroxybutyrate were viable upon transfer to recipients, although no pregnancies were confirmed later by ultrasonic scanning. The protective effect of serum upon embryos cultured in medium containing acetoacetate is apparently not required in the presence of D-beta-hydroxybutyrate.

Published

2002

17. Culture system and long-term storage of culture media in the in vitro production of bovine embryos

Author

C.O. Hidalgo, Adelino Katchicualula, Carolina Tamargo, M. Carbajo, Santiago de la Varga, L. Fernandez, Carmen Díez, and Jenny Álvarez

Subjects

Fetus, General Veterinary, business.industry, Hatching, Embryogenesis, Fertilization in Vitro, Biology, Cryopreservation, Biotechnology, Culture Media, Andrology, Embryo Culture Techniques, chemistry.chemical_compound, medicine.anatomical_structure, chemistry, Sodium citrate, biology.protein, medicine, Oocytes, Oviduct, Animals, Cattle, Blastocyst, Bovine serum albumin, business

Abstract

The optimum culture system for in vitro matured and fertilised oocytes still remains to be clarified. Culture media (CM) for mammalian embryos are routinely prepared fresh for use and preserved under refrigeration during one or two weeks. The purposes of this work were (1) to compare the efficiency of a synthetic oviduct fluid (SOF) with two different bovine serum albumin (BSA) concentrations (3 and 8 g/L) for the in vitro production of bovine blastocysts, (2) to test the effect of timing on adding fetal calf serum (FCS) to the SOF, and (3) to evaluate the effects on bovine embryo development of freezing and lyophilisation as procedures for preserving the SOF. Supplementation of SOF with 3 g/L BSA increased Day-7 blastocyst expansion rates (18.3 ± 1.6 vs. 14.4 ± 0.7; P < 0.05), although no differences in hatching rates were found. Addition of FCS to SOFaa (SOF with amino acids) medium supplemented with sodium citrate (SOFaaci) at 48 and at 72 h post-insemination (PI) allowed obtaining higher Day-6 embryo development rates than when FCS was added at 18 or 96 h PI (Day-6 morulae + blastocyst rate: 30.0 ± 1.1, 40.8 ± 1.1, 43.9 ± 2.3 and 39.3 ± 0.5 for FCS addition at 18, 48, 72 and 96 h, respectively). Hatching rates were significantly improved when serum was added at 72 h PI. Finally, both refrigeration and lyophilisation appeared as useful cryopreservation procedures for SOFaaci, although a significant loss of its ability to support embryo development, compared to the control fresh culture medium, was observed.

Published

2011

18. Programa de conservación del Gochu Astur-Celta: creación de un banco de germoplasma

Author

Aurelio Rodríguez, C. Tamargo, M.J. Merino, J. M. Benito, A. Fernández, C.O. Hidalgo, and M.J. Reyes

Subjects

Razas autóctonas, Male fertility, media_common.quotation_subject, Animal Science and Zoology, Forestry, Espermatozoide, Verraco, Reproduction, Biology, media_common, Crioconservación

Abstract

El objetivo de este trabajo fue el estudio de la posibilidad de criopreservar semen de verracos de la raza porcina autóctona Gochu Astur-Celta, que en la actualidad se encuentra en peligro de extinción, como herramienta en los planes de recuperación de la raza. Las dosis seminales obtenidas a partir de los eyaculados recogidos fueron envasadas, sometidas a congelación y posteriormente almacenadas en nitrógeno líquido, analizándose los siguientes parámetros: motilidad y calidad del movimiento, integridad funcional de la membrana, morfología y estado del acrosoma. Los resultados obtenidos muestran que es necesario seguir trabajando en la mejora de la calidad del semen congelado-descongelado para que esta técnica pueda contribuir a la conservación de la biodiversidad.

Published

2011

19. Serum free embryo culture medium improves in vitro survival of bovine blastocysts to vitrification

Author

Marta Muñoz, Aurelio Rodríguez, C.O. Hidalgo, Carmen Díez, N. Facal, Enrique J. Gómez, E. Moran, and José Néstor Caamaño

Subjects

Male, animal structures, Embryonic Development, Fertilization in Vitro, Culture Media, Serum-Free, Andrology, Embryo Culture Techniques, Food Animals, Chlorocebus aethiops, Animals, Vitrification, Small Animals, Vero Cells, Cryopreservation, Equine, Chemistry, Embryogenesis, Embryo culture, Embryo, Serum Albumin, Bovine, Embryo, Mammalian, Embryo transfer, Coculture Techniques, In vitro maturation, Blastocyst, embryonic structures, Immunology, Vero cell, Oviduct, Animal Science and Zoology, Cattle, Female

Abstract

The aim of this study was to examine the effects of co-culture with Vero cells during the in vitro maturation (IVM) and three culture media, B2+5% fetal calf serum (FCS) on Vero cells, synthetic oviduct fluid (SOF)+5% FCS, and SOF+20gL −1 bovine serum albumin (BSA), on the developmental competence of the embryos and their ability to survive vitrification/warming. We also tested the effect of morphological quality and the age of the embryo on its sensitivity to vitrification. The IVM system neither affects the embryo development up to Day 7 nor survival rates after vitrification. The culture of embryos in SOF+FCS and in Vero cells+B2 allowed obtaining more Day 6 and Day 7 blastocysts, and a higher % of Day 7 blastocysts vitrified than culture in SOF+BSA. Contrarily, on Day 8, more blastocysts were vitrified in SOF+BSA than in SOF+FCS. Blastocysts quality affected development after vitrification/warming, and Day 7 embryos showed higher survival rates than their Day 8 counterparts. Day 7 blastocysts produced in Vero cells or in SOF+BSA survived at higher rates than those produced in SOF+FCS at 24 and 48h after warming. Embryo culture with BSA allows obtaining hatching rates after vitrification/warming higher than those obtained after co-culture with Vero cells in B2 and FCS. Moreover, this system provides hatching rates from Day 8 blastocysts comparable to those obtained on Day 7 in Vero cells. Further studies, including embryo transfer to recipients, are needed to clarify factors affecting the freezability of in vitro produced bovine embryos.

Published

2007

20. Effects of re-infection with Neospora caninum in bulls on parasite detection in semen and blood and immunological responses

Author

C.O. Hidalgo, Luis Miguel Ortega-Mora, I. del-Pozo, A. Martínez, G. Aduriz, Enrique Serrano-Martínez, A. Mateos-Sanz, Koldo Osoro, C. Tamargo, and Ignacio Ferre

Subjects

Male, endocrine system, Time Factors, animal diseases, Cattle Diseases, Mice, Nude, Semen, Parasite load, Andrology, Mice, fluids and secretions, Immune system, Food Animals, Recurrence, parasitic diseases, Parasite hosting, Animals, Seroconversion, Small Animals, Mice, Inbred BALB C, biology, urogenital system, Equine, Inoculation, Coccidiosis, Immunity, Neospora, DNA, Protozoan, biology.organism_classification, Virology, Neospora caninum, Protozoa, Animal Science and Zoology, Cattle, Female

Abstract

Three bulls with experimentally induced primary infection with Neospora caninum were re-infected intravenously with 10 8 live N. caninum tachyzoites of the NC-1 isolate at 300 days post-infection to investigate the presence of N. caninum in semen and blood, and the associated immune responses. In parallel, three bulls with experimentally induced primary infection with N. caninum and three non-infected bulls were also monitored. Re-infected and infected bulls showed an intermittent presence of N. caninum DNA in semen with a parasite load ranging from 0.1 to 15.6 (mean 4.4) and 0.1 to 11.1 (mean 4.1) parasites/ml, respectively. Re-infected bulls showed significant and persistent serum-specific IgM and IgG antibody responses. Specific IgG levels were detected in seminal plasma of all infected bulls, but the magnitude of the response was significantly higher in re-infected rather than in chronically infected animals. The mean specific IFN-γ levels in re-infected bulls were significantly increased as early as 3 and 7 days after experimental infection when compared to bulls in other groups. This study showed that the intermittent presence and parasite load of N. caninum in the semen of re-infected bulls is very similar to that reported in chronically infected animals. The protozoa could not be isolated from BALB/c nu/nu mice inoculated with PCR-positive semen samples and inseminated heifers with pooled semen samples did not show seroconversion. Plasma IFN-γ level seems to be a good indicator of a recent N. caninum infection.

Published

2007

21. Intrauterine Neospora caninum inoculation of heifers and cows using contaminated semen with different numbers of tachyzoites

Author

R.A. Mota, Luis Miguel Ortega-Mora, Enrique Serrano-Martínez, A. Martínez, Ignacio Ferre, C.O. Hidalgo, G. Aduriz, I. del-Pozo, and Koldo Osoro

Subjects

Time Factors, Pregnancy Rate, medicine.medical_treatment, Antibodies, Protozoan, Cattle Diseases, Semen, Biology, Insemination, Serology, Interferon-gamma, Animal science, Neospora, Food Animals, Pregnancy, medicine, Animals, Seroconversion, Small Animals, Uterine Diseases, Equine, Coccidiosis, Artificial insemination, DNA, Protozoan, biology.organism_classification, Neospora caninum, Pregnancy rate, Pregnancy Complications, Parasitic, Animal Science and Zoology, Cattle, Female

Abstract

Objective To investigate the potential of different Neospora caninum tachyzoite doses to infect heifers (experiment 1) and cows (experiment 2) when administered in utero by artificial insemination via contaminated semen. Methods In experiment 1, five groups of 5, 7, 8, 9, and 5 cyclic heifers were hormonally synchronized and artificially inseminated with semen containing 0 (A, controls), 102 (B), 5 × 103 (C), 5 × 104 (D), and 5 × 105 (E) live N. caninum NC-1 isolate-tachyzoites, respectively. Experimental infection was followed for 100 days. Parasitaemia and specific serum IgG, and interferon-gamma (IFN-γ) responses were studied. In experiment 2, four groups of 9, 10, 9, and 9 adult multiparous cows with confirmed infertility problems of diverse aethiology were hormonally synchronized and artificially inseminated with semen containing 0 (a, controls), 102 (b), 5 × 103 (c), and 5 × 105 (d) live N. caninum NC-1 isolate-tachyzoites, respectively. Experimental infection was followed for 63 days. Parasitaemia and specific serum IgG responses were studied. Results In experiment 1, parasitaemia was detected in 1, 2, and 3 heifers from groups B, C, and D, respectively, between 9 and 23 days after insemination. Persistent specific serum antibody responses were detected in 2 and 3 heifers from groups D and E, respectively. Transient specific serum antibody responses were detected in 2, 1 and 1 heifers from groups C, D, and E, respectively. In addition, 1 heifer from group B showed a serum-specific antibody level higher than cut off value at 21 days post-insemination. Heifers seroconverted between 23 and 47 days after insemination. Specific IFN-γ levels were detected in 1, 4, 6, and 3 heifers from groups B, C, D, and E, respectively, between 9 and 55 days after insemination. Pregnancy rate in the control group (60%) was higher than those observed in inoculated heifers (0–42.9%). Pregnancy rates in inoculated heifers were lower when the tachyzoite dose was increased (B 42.9%, C 12.5%, D 11.1%, and E 0%). In experiment 2, no Neospora DNA in blood nor specific serum IgG to N. caninum were detected in any of the cows studied, except in one cow inoculated with 5 × 105 tachyzoites (group d) which showed a relative index × 100 (RIPC) values of 9.4, 18.9, and 18.1 at 42, 56, and 63 days after insemination, respectively. Conclusions This study provides evidence that the intrauterine infection via contaminated semen using 5 × 104 and 5 × 105 tachyzoites caused persistent serum-specific antibody responses in some heifers. On the basis of serological data, a dose–response effect was also observed. In addition, N. caninum would be a probable cause of early foetal death in inoculated heifers. In contrast, results obtained in a similar experiment with cows showing confirmed infertility indicate that higher doses, such as of 5 × 105 tachyzoites, were necessary to induce seroconversion in at least one animal.

Published

2006

22. Oocytes recovered from cows treated with retinol become unviable as blastocysts produced in vitro

Author

P. Duque, N. Facal, C. Alonso-Montes, Félix Goyache, Shuntaro Ikeda, Enrique J. Gómez, Aida Rodríguez, Carmen Díez, C.O. Hidalgo, J.M. Prendes, and Iván Sánchez Fernández

Subjects

Vitamin, Male, Embryology, medicine.medical_specialty, Time Factors, genetic structures, Cell Survival, Retinoic acid, Tretinoin, Fertilization in Vitro, Biology, Morula, Follicle, chemistry.chemical_compound, Endocrinology, Internal medicine, medicine, Animals, Blastocyst, Vitamin A, Retinol, Obstetrics and Gynecology, Embryo, Cell Biology, Oocyte, Embryo Transfer, Follicular fluid, Follicular Fluid, medicine.anatomical_structure, Teratogens, Reproductive Medicine, chemistry, Oocytes, Cattle, Female

Abstract

Retinoids have been shown to enhance developmental competence of the oocyte in cattle, sheep and pigs. In this study we investigated whether exogenous retinol stimulates the bovine oocyte during its intrafollicular growth and the time limits of exposure to exogenous retinol. In addition, we also determined the efficiency of ovum pick-up techniques in combination with retinol treatment and the viability of embryos after transfer to recipients. In Experiment 1, heifers were injected with retinol or vehicle, and concentrations of retinol in the blood were analysed on Day 0 (prior to injection), Day 1 and, together with follicular fluid, Day 4. Blood retinol increased by Day 1 and cleared on Day 4, but retinol remained higher within the follicle. In Experiment 2, oocyte donors were injected weekly with retinol or vehicle four times during a twice-per-week cycle of eight recovery sessions (starting 4 days before the first session), followed by a second eight-session cycle without treatment. Oocytes recovered were fertilized and culturedin vitro.Retinol treatment yielded higher numbers of low-quality oocytes throughout, although retinol measured during cycles did not change. Total oocytes, and morulae and blastocyst rates, increased during the first five sessions following treatment with retinol. As previously shown with oocytes from slaughterhouse ovaries, retinoic acid stimulated blastocyst development. Following transfer to recipients, blastocysts from oocytes exposed to retinol were unable to establish pregnancy. Our study confirms the existence of an effect of retinol on the intrafollicular oocyte in the cow and provides evidence regarding the teratogenic effect of retinol.

Published

2005

23. Bovine oocyte vitrification before or after meiotic arrest: effects on ultrastructure and developmental ability

Author

C.O. Hidalgo, Santiago de la Varga, Alba Fernández, N. Facal, L. Fernandez, Carolina Tamargo, P. Duque, Carmen Díez, M. Carbajo, Aida Rodríguez, and Enrique J. Gómez

Subjects

Cytoplasm, Fertilization in Vitro, Cryopreservation, Andrology, Embryo Culture Techniques, Food Animals, Ovarian Follicle, medicine, Animals, Vitrification, Small Animals, Cells, Cultured, Cell Nucleus, Estradiol, urogenital system, Equine, Chemistry, Embryo, Luteinizing Hormone, Oocyte, In vitro maturation, Culture Media, Meiosis, Microscopy, Electron, medicine.anatomical_structure, Bovine oocyte, Meiotic arrest, Ultrastructure, Oocytes, Animal Science and Zoology, Cattle, Female, Follicle Stimulating Hormone

Abstract

The nuclear stage at which oocytes are cryopreserved influences further development ability and cryopreservation affects ultrastructure of both cumulus cells and the oocyte. In this work, we analyze the effects of vitrification at different nuclear and cytoplasmic maturation stages on the oocyte ultrastructure and developmental ability. Culture in TCM199 + PVA with roscovitine 25 M during 24 h led to meiotic arrest (MA) in cumulus-oocyte complexes (COCs), while permissive in vitro maturation (IVM) was performed in TCM199, 10% FCS, FSH-LH and 17β-estradiol for 24 h. Oocytes were vitrified using the open pulled straw method (OPS) with minor modifications. Fresh and vitrified/warmed COCs were fixed as immature, after IVM, after meiotic arrest (MA) and after MA + IVM. Vitrification combined with MA followed by IVM produced the highest rates of degeneration, regardless of the vitrification time. As a consequence, lower proportions of embryos cleaved in these groups, although differences were eliminated at the five–eight cell stage. Development rates up to day 8 were similar in all experimental groups, being significantly lower than those in fresh controls. Only oocytes vitrified after IVM were able to give blastociysts. The morphological alterations observed can be responsible for compromised development. More research is needed to explain the low survival rates of the bovine oocyte after vitrification and warming.

Published

2004

24. Macromolecular source as dependent on osmotic pressure and water source: effects on bovine in vitro embryo development and quality

Author

Belén Pintado, C.O. Hidalgo, Carmen Díez, Enrique J. Gómez, N. Facal, and P. Duque

Subjects

Embryology, cell number, Medicine (miscellaneous), water quality, 0302 clinical medicine, Inner cell mass, Osmotic pressure, Bovine serum albumin, osmolarity, [SDV.BDD]Life Sciences [q-bio]/Development Biology, 030219 obstetrics & reproductive medicine, biology, in vitro produced bovine embryo, Cell Differentiation, Serum Albumin, Bovine, 04 agricultural and veterinary sciences, medicine.anatomical_structure, Biochemistry, embryonic structures, Female, Cell Division, Serum albumin, Fertilization in Vitro, Andrology, 03 medical and health sciences, Embryonic and Fetal Development, Osmotic Pressure, Culture Techniques, medicine, Animals, Blastocyst, Osmole, Osmotic concentration, 0402 animal and dairy science, Water, Embryo culture, [SDV.BDLR]Life Sciences [q-bio]/Reproductive Biology, 040201 dairy & animal science, Culture Media, Embryo Research, Reproductive Medicine, Polyvinyl Alcohol, biology.protein, Animal Science and Zoology, Cattle, protein, [SDV.AEN]Life Sciences [q-bio]/Food and Nutrition, Developmental Biology, Food Science

Abstract

International audience; This study evaluated the protective effect of protein, as dependent on osmolarity, and the quality of water sources used to prepare embryo culture media. In Experiment 1, two concentrations of NaCl were used to obtain culture media with normal (280 mOSM) and low (245 mOSM) osmolarity, each supplemented with either bovine serum albumin (BSA) or polyvinyl alcohol (PVA). Low osmolarity improved blastocyst rates in the presence of BSA ($P < 0.01$) and tended to do it in medium containing PVA ($P < 0.07$). Furthermore, low osmolarity allowed PVA to increase inner cell mass (ICM) numbers and ICM/total cell rate ($P < 0.05$), while trophectoderm (TE) and total cell counts tended to decrease ($P < 0.08$). In Experiment 2, culture media were prepared with two water sources (Milli-Q and Sigma-W3500-) in combination with BSA or PVA. Both water sources yielded similar embryo development rates, but in the presence of BSA, Milli-Q water produced embryos with increased ICM/total cells rates ($P < 0.05$). On the contrary, Sigma water tended to increase trophectoderm cell counts ($P < 0.08$). In conclusion, the present study showed that low osmolarity is beneficial to embryo development and combinations of macromolecule and osmolarity influence trophectoderm differentiation. Both Milli-Q and Sigma supported embryo development at comparable rates, although in the presence of BSA, blastocysts obtained in the medium prepared with Milli-Q water had superior quality in terms of ICM/total cells rates.

Published

2004

25. Enhancement of developmental capacity of meiotically inhibited bovine oocytes by retinoic acid

Author

Gustavo Ferrer Carneiro, P. Duque, Luis J. Royo, Pedro Lorenzo, Carmen Díez, C.O. Hidalgo, N. Facal, and Enrique J. Gómez

Subjects

Cytoplasm, Retinoic acid, Cortical granule, Cell Count, Tretinoin, Fertilization in Vitro, Biology, chemistry.chemical_compound, Culture Techniques, medicine, Animals, Blastocyst, Cells, Cultured, Fallopian Tubes, Fluorescent Dyes, Cryopreservation, Microscopy, Confocal, Rehabilitation, Embryogenesis, Retinol, Obstetrics and Gynecology, Embryo, Oocyte, Cell biology, Body Fluids, Meiosis, medicine.anatomical_structure, Reproductive Medicine, chemistry, Microscopy, Fluorescence, Immunology, Oocytes, Cattle, Female, medicine.drug

Abstract

BACKGROUND Although high vitamin A may be teratogenic to the embryo, retinol has been shown to support oocyte developmental potential in vivo. Similarly, addition of retinol metabolite 9-cis-retinoic acid to in-vitro cultured oocytes could promote cytoplasmic maturation and subsequent early embryonic development. The objective of this study was to evaluate the effects of 5 nmol/l retinoic acid during in-vitro pre-maturation and maturation of bovine oocyte-cumulus complexes. METHODS AND RESULTS Oocytes were aspirated from cows and either kept under meiotic arrest with 25 micro mol/l roscovitine and matured, or allowed to mature in permissive conditions (control). Cortical granule migration was analysed both after pre-maturation and maturation by fluorescent labelling of oocytes and subsequent laser confocal and fluorescence microscopy. Variables studied after in-vitro fertilization and culture in modified synthetic oviduct fluid were: (i) in-vitro embryonic development; (ii) ability of blastocysts to survive vitrification and warming; and (iii) differential cell counts measured by fluorescence microscopy. Although the presence of 5 nmol/l retinoic acid throughout in-vitro maturation was harmful, its presence during pre-maturation alone improved cytoplasmic granular migration, embryonic development, cryopreservation tolerance, total cell numbers and, as a consequence, embryonic quality. CONCLUSIONS Pre-maturation in the presence of retinoic acid improves cytoplasmic competence of in-vitro matured bovine oocytes. Until more is known of the molecular mechanisms it would be irresponsible to use retinoic acid in maturation of human oocytes, especially in view of the narrow time window and possible species-specific differences in susceptibility and protection of the oocyte from epigenetic influences of retinol.

Published

2002

26. 162 FREEZING OF SEMEN FROM ENDANGERED ASTURIANA DE LA MONTAÑA BULLS IN ZWITTERONIC LIPIDS-BASED EXTENDERS

Author

Aurelio Rodríguez, C.O. Hidalgo, A.T. Palasz, P. Beltrán Breña, S. S. Pérez-Garnelo, C. Tamargo Miguel, and J. de la Fuente

Subjects

medicine.diagnostic_test, urogenital system, Extender, Cold storage, Semen, Anatomy, Reproductive technology, Biology, Semen analysis, Sperm, Cryopreservation, law.invention, Endocrinology, Animal science, Reproductive Medicine, law, Genetics, medicine, Animal Science and Zoology, Molecular Biology, Sperm motility, Developmental Biology, Biotechnology

Abstract

This experiment was designed to test the efficacy of 2 different preparation protocols of zwitteronic soyabean-origin lipids for the production of lipidsglycerol liposomes for use in bull semen cryopreservation. Lipids liposomes were prepared at 10% concentration in Tris buffer by 1. highpressure homogenization (Panda 2K, Parma, Italy) and then 8% glycerol were added, extender-1 (E-1); Lipids were homogenized together with glycerol, extender-2 (E-2). Bioxcell extender (E-3) was used as control. Semen was collected 3 times from 3 endangered Asturiana de la Monta�a bulls by the means of an artificial vagina. Ejaculates with at least 70% motility were processed further by a standard freezing protocol used in our AI station. Semen was diluted at 37�C with each of the 4 extenders to a concentration of 92 � 106 spermatozoa per mL, cooled to 4�C over 4 h, aspirated into 0.25-mL plastic straws (IMV Technologies, Aigle, France), frozen in a bio-freezer (IMV Technologies) in 3 steps from 4 to –140�C, and then plunged into liquid N2. Straws were thawed in a water bath at 37�C for 30 s. Sperm motility was analyzed microscopically immediately after collection, after dilution, and after 4, 24, 48, and 72 h of storage at 4�C. Post-thaw semen progressive motility was assessed microscopically, and sperm movement characteristics were analyzed by computer-assisted semen analysis (CASA) (SCA�, Microptic, Barcelona, Spain). Data were compared between extenders and bulls by 2-way ANOVA; percentages were transformed by arcsine transformation before ANOVA. Total and progressive sperm motility at 0 h after dilution ranged from 90 to 70% and was not different between extenders and bulls. There was no difference between bulls in total and progressive motility after 24 h of cold storage; however, both were significantly greater (P < 0.05) for Control (62.4 � 14.7 and 41.4 � 14.9) and E-1 (70.1 � 12 and 33.8 � 7.0) extenders than for the E-2 extender (22.5 � 17 and 1.2 � 1.3). Average post-thaw sperm motility was not different between bulls for either extender, but motility for Bioxcell (Control, 48.1 � 14.6%) and E-1 extenders (43.2 � 13.0%) were significantly greater (P < 0.05) than for E-2 extender (18.7 � 8.8%). There were no differences between bulls for all kinematic semen parameters: curvilinear (VCL), straight line (VSL), average path (VAP) velocities, linearity (LIN) and straightness (STR), evaluated by CASA before and after freezing; however, all were lower (P < 0.05) for the E-2 extender and not different between Control and E-1 extenders. Sperm movements derived from heads (VCL) and linearity of sperm(LIN), both closely related to field fertility, were in the range of 90.9 � 2.1 and 63.0 � 5.5 for E-3 (Control) extender; 99.1 � 3.4 and 49.4 � 3.5 for E-1; and 21.8 � 2.2 and 29.9 � 4.0 for E-2. In summary, zwitteronic soyabean lipid liposomes are an effective egg yolk substitute for the cryopreservation of Asturiana de la Monta�a bull semen; however, the homogenization protocol of the lipids-glycerol mixture must be improved.

Published

2008

27. 20 SPERM CHARACTERIZATION OF ASTURCON PONIES AFTER COLLECTION AND EQUILIBRATION/REFRIGERATION BEFORE FREEZING

Author

J. M. Benito, C. Tamargo, J. de la Fuente, M. Carbajo, C.O. Hidalgo, and Carmen Díez

Subjects

urogenital system, Extender, Semen, Reproductive technology, Anatomy, Biology, Sperm, Breed, law.invention, Semen quality, Endocrinology, Animal science, Reproductive Medicine, law, Reproductive biology, Genetics, Animal Science and Zoology, Molecular Biology, Sperm motility, Developmental Biology, Biotechnology

Abstract

The need to conserve farm animal biodiversity is accepted by many countries through the ratification of the convention of biological diversity, and sperm quality is known to be an important criterion in the evaluation of breeding soundness. The aim of this work was to characterize the semen of a local breed of ponies 'Asturcon' (maintained free over the mountains all year around) before its incorporation into a germplasm bank. Semen was obtained from six stallions (6–17 years of age) using an artificial vagina, 3 days/week, during 12 weeks. Immediately after collection, gel-free semen was evaluated for volume, sperm concentration, and motility. Semen motility was again evaluated after equilibration/refrigeration. For evaluation of individual (IM) and progressive motility (PM) rates, semen was diluted (20 � 106 spermatozoa/mL) and analyzed with a CASA System (SCA; Microptic S.L., Barcelona, Spain). Five fields per sample were evaluated (minimum 500 spermatozoa/sample) under a phase contrast microscope (100�). Semen samples were subjected to a hypo-osmotic swelling test (HOS) test to detect the presence of swollen tails in a 100 mM citrate–fructose solution. Percentages of altered acrosomes and morphological abnormalities were determined by counting 100 spermatozoa (1000�). Then, semen was diluted and centrifuged for 10 min at 600g. After the supernatant was discarded, the pellet was re-suspended in freezing medium (skim milk extender containing 2% egg yolk and 2.5% glycerol) to a final concentration of 100 � 106 spermatozoa/mL, and equilibrated/cooled (60 min) to 4�C. Statistical analysis was carried out by means of the GLM and CORR procedures and Duncan test for means (SAS Institute, Inc., Cary, NC, USA). A significant effect between males (P < 0.05) on semen quality, such as volume of the ejaculate, sperm concentration, and morphological abnormalities, were detected among stallions. On the other hand, positive and significant correlations were found between the sperm motility immediately after collection and after equilbration/refrigeration (r = 0.73; P < 0.05); moreover, sperm motilities (both fresh and refrigerated) correlated with the results of the HOS test (r = 0.56; P < 0.001, and r = 0.27, P < 0.05, respectively). These preliminary results confirm that the sperm of the Asturcon ponies breed can be collected and will survive the equilibration/refrigeration procedures. Conservation and development of local breeds is important because they represent a unique source of genes for improving health and performance traits of industrial breeds. However, complementary studies on the ability of the stallion sperm to survive freezing/thawing procedures in rates higher than 30% are needed to ensure that genetic banks are correctly created. This work was performed in collaboration with ACPRA and Dep�sito de Sementales de Santander (Spain), and supported by RZ2004-00031-C02-01.

Published

2007

28. 111 ESTIMATION OF SPERM QUALITY IN FRESH AND FROZEN - THAWED SEMEN FROM ASTURIANA DE LOS VALLES BULLS

Author

D. Martin, C.O. Hidalgo, Carmen Díez, M. Carbajo, and C. Tamargo

Subjects

urogenital system, Artificial insemination, medicine.medical_treatment, Semen, Anatomy, Reproductive technology, Biology, Semen cryopreservation, Sperm, Andrology, Semen quality, Endocrinology, Reproductive Medicine, Genetics, medicine, Animal Science and Zoology, Molecular Biology, Spermatogenesis, Sperm motility, Developmental Biology, Biotechnology

Abstract

Artificial insemination and semen cryopreservation have significantly improved the breeding potential of male animals. However, current freezing techniques commonly result in reduced semen quality (Januskauskas et al. 1999 Theriogenology 52, 641-658), and surviving cells are affected post-thaw either structurally or functionally (Nagy et al. 2004 Anim. Reprod. Sci. 80, 225-235). In this work we analyze the impact of cryopreservation on Asturiana de los Valles bull sperm. Ejaculates (n = 373) from seven adult bulls were weekly collected by means of artificial vagina. Immediately after collection, routine parameters including volume (V), mass motility (MM), and concentration (C) of sperm cells were evaluated. Then the semen was extended with a commercial extender, loaded into 0.25-mL plastic straws at a concentration of 23 � 106 per straw, frozen and stored for further analysis. Four straws per ejaculate were thawed, pooled and analyzed for motion characteristics by means of a CASA system (Sperm Class Analyzer, SCA 2002� Microptic S. L., Barcelona, Spain) added to an optical phase-contrast microscope with heatable (37�C) stage. Immediately after thawing, we analyzed the % of motile spermatozoa (MS) and the % of progressively motile spermatozoa (PMS); then samples were incubated for 3 h at 37�C and MS and PMS were measured again (MS3 and PMS3, respectively). Functional integrity of the plasmallema was evaluated by the hypoosmotic swelling test (HOST) together with the % of typical tail coiling/swelling (percentage of HOST-positive spermatozoa, HOST-PS). The % of viable spermatozoa (VS) [membrane integrity was evaluated by fluorescence microscopy with a dual staining system (propidium iodide (PI) and 6-carboxyfluorescein diacetate (CFDA)]. Sperm showing partial or complete red fluorescence (PI staining) were considered nonviable, whereas sperm showing complete green fluorescence were considered viable. Altered acrosomes (AA) and morphological abnormalities were also determined. The % of morphological abnormalities was classified according to their location in head (HA), midpiece (MA), and tail (TA). Proximal and distal cytoplasmic droplets were counted as separate abnormalities (CD). Data were analyzed by the MEANS procedure of SAS (SAS Institute, Inc., Cary, NC, USA). A significant (P < 0.05) decrease in the sperm motility was observed after freezing/thawing (MS: 80.20 � 0.75 vs. 47.36 � 1.04, and PMS: 68.73 � 0.73 vs. 42.14 � 0.96 for fresh and frozen-thawed semen, respectively). Also, the frozen-thawed sperm showed increased % of HA, MA, AA, HOST-PS, and VS (P < 0.05). These morphological abnormalities could contribute to decreasing sperm motility. The new computer and video technologies provide useful information about sperm quality and can be used in the daily routine of processing semen. This work was performed in collaboration with ASEAVA.

Published

2006

29. 205 DEVELOPMENT OF OOCYTES FROM COWS TREATED WITH RETINOL IS COMPROMISED PRIOR TO IMPLANTATION

Author

Carmen Díez, N. Facal, E. Moran, Aida Rodríguez, Shuntaro Ikeda, C. Alonso-Montes, C.O. Hidalgo, J.M. Prendes, and Enrique J. Gómez

Subjects

Estrous cycle, medicine.medical_specialty, Theriogenology, Embryo culture, Reproductive technology, Biology, Embryo transfer, Andrology, Follicle, Endocrinology, Reproductive Medicine, Immunology, Genetics, medicine, Animal Science and Zoology, Folliculogenesis, Molecular Biology, Spermatogenesis, Developmental Biology, Biotechnology

Abstract

In the cow, sheep, and gilt, a retinoid support enhances the oocyte development (reviewed by Hidalgo C et al. 2003 Reproduction 125, 409–416). The shortest effective time interval for these animals injected with retinol (ROH) is four days, but the reasons for this have not been described. Furthermore, the development after transfer of embryos derived from oocytes of donors treated with ROH is not known. The objective of the present work was to elucidate the two above questions. We analyzed the ROH and retinyl palmitate (REP) contents in plasma and follicular fluid (FF). The estrus cycles of heifers (n = 12) were synchronized with progestagen and PGF2α. Blood samples were taken at progestagen removal (Day 0). Animals were injected with 1 × 106 ROH units (n = 6) or corn oil (vehicle; n = 6) on Days 0, 1, and 4. Contents of follicles between 3 and 10 mm were aspirated on Day 4 by an ultrasound-guided procedure. All samples were analyzed for ROH and REP by HPLC. To produce embryos for transfer, follicles were aspirated from donors treated four times with 1 × 106 ROH units/week or vehicle, starting four days before the first aspiration. Both groups of cumulus-oocyte complexes (COCs) were matured in vitro with or without 5 nM 9-cis-retinoic acid (RA). The presence of RA prolonged the exposure to retinoids (cows treated with ROH) or acted as a positive control (heifers with vehicle). Oocytes were fertilized and cultured in mSOF + 5% FCS. Embryo transfer (ET) to recipients was performed with fresh (one) or vitrified (two) good-morphology Day 7 embryos, and pregnancy monitored on Days 21, 35, and 60. Data analysis was by GLM (ROH and REP concentrations) or CATMOD (pregnancy monitoring), and Duncan's test (a,bP < 0.05; v,x,y,zP < 0.02). Average FF volume recovered were 351 ± 127 μL (controls; range 100–700) and 393 ± 127 μL (ROH; range 80–950). Concentrations of REP were unaffected by timing, follicle or blood, and ROH treatment (data not shown). Concentrations of ROH (μg/dL) for vehicle and ROH-treated cows were (LSM ± SE) 42.0 ± 1.8vx and 42.0 ± 2.4vx (plasma-Day 0, before ROH injection), 37.3 ± 1.8v and 47.64 ± 2.4x (plasma-Day 1), 42.6 ± 1.9vx and 45.5 ± 2.3vx (plasma-Day 4), and 6.1 ± 3.0y and 16.8 ± 2.6z (FF-day 4), respectively. Cumulatively, embryos from donors receiving ROH did not exhibit pregnancy on Day 21 (0/15x; confirmed on Day 35), which differed from vehicle donors on Day 21 (44%, 8/18y) and Day 35 (33%, 6/18y), and tended to differ (P = 0.07) on Day 60 (22%, 4/18). Pregnancy rates were independent of fresh or vitrified embryos within ETs. Injected ROH elevated blood concentrations of ROH, although values became normalized on Day 4. However, a coasting period of 4 days for ROH administration seems to be justified by increased intrafollicular levels of ROH. Development into blastocysts is disrupted before implantation, showing that ROH directly affects the oocyte during its intrafollicular growth. This work was supported by MCYT-AGL-2002-0117.

Published

2005

30. 128CHANGES WITHIN OXYGEN ENVIRONMENT DURING IVF AND IVC IMPROVE BOVINE EMBRYONIC DEVELOPMENT IN VITRO

Author

B. Marquant-Le Guienne, Enrique J. Gómez, P. Humblot, N. Facal, Carmen Díez, C.O. Hidalgo, J.M. Prendes, and E. Moran

Subjects

medicine.medical_specialty, Theriogenology, Embryo culture, Anatomy, Reproductive technology, Biology, Sperm, Cryopreservation, Oxygen tension, Andrology, Endocrinology, medicine.anatomical_structure, Reproductive Medicine, Genetics, medicine, Animal Science and Zoology, Blastocyst, Molecular Biology, Spermatogenesis, Developmental Biology, Biotechnology

Abstract

Oxygen concentration during both IVF and IVC affects embryonic development. A low O2 atmosphere during IVC has been reported to be beneficial for embryos in culture without somatic cells. Similarly, a reduction in spermatozoa (sp) concentration can influence the oxygenation grade of fertilization medium, and O2 requirements can vary according to the embryonic stage of development. This experiment investigated whether prolonged contact with sperm cells interacts with effects of oxygen tension during the first days of culture. Slaughterhouse bovine COCs matured with Vero-cells in TCM199 with FCS and EGF were co-incubated (CI) with swim-up separated sp. COCs with attached sp were either removed after 2h and placed in IVF medium without sp up to completion of 18h (sp-restricted CI), or COCs and sp were left together for 18h (sp-prolonged CI). Zygotes were cultured in serum-free, B2 medium conditioned with Vero cells (Marquant-Le Guienne et al., 1999 Theriogenology 51, 386), modified as described by Gomez and Diez (2000 Anim. Reprod. Sci. 58, 23–37). According to IVF procedure (sp-restricted or sp-prolonged), embryo culture was made either in 20% O2 from Day 0 up to Day 3 and in 5% O2 later on, or in 5% O2 from Day 0 up to Day 8, in a 2×2 factorial design. IVF medium was monitored for Na+, K+, Ca2+, pH, O2, CO2 , HCO3− and lactate (i-STAT analyzer; 5 replicates -R-) at 0h, 2h and 18h without cells (controls), at 2h in CI and at 18h both in sp-restricted and sp-prolonged CI. Embryo development was analyzed by CATMOD for effects, and all data were processed by GLM and Duncan test and expressed as LSM±SE. The presence of cells decreased pO2 (P

Published

2004

31. 112EFFECT OF THE IVM PROTOCOL OF BOVINE OOCYTES ON SURVIVAL RATES AFTER VITRIFICATION BY OPEN PULLED STRAW METHOD

Author

Carmen Díez, N. Facal, E. Moran, Enrique J. Gómez, C.O. Hidalgo, and Aida Rodríguez

Subjects

Embryo culture, Reproductive technology, Anatomy, Biology, Oocyte, Oogenesis, Cryopreservation, In vitro maturation, Andrology, Endocrinology, medicine.anatomical_structure, Reproductive Medicine, Genetics, medicine, lipids (amino acids, peptides, and proteins), Animal Science and Zoology, Folliculogenesis, Blastocyst, Molecular Biology, Developmental Biology, Biotechnology

Abstract

The meiotic stage and the cryopreservation protocol influence the ability of the oocytes to survive cryopreservation. The in vitro maturation (IVM) methods affect nuclear and cytoplasmic maturation and, consequently, the developmental competence of the oocytes. On the other hand, the cytoplasm of the bovine oocyte contains large amounts of lipids which, as demonstrated in the bovine embryo (Díez et al., 2001 Theriogenology 55; 923–936), can negatively affect post-thaw survival. The aim of this work was to analyze the effect of fetal calf serum (FCS) during IVM on the freezability of the bovine metaphase II oocyte. Cumulus-oocyte complexes (COCs) were recovered from slaughterhouse ovaries. Oocytes with compact cumulus cells and evenly granulated cytoplasm were matured for 22h in TCM199, NaHCO3, FSH, LH and 17βestradiol. Approximately half of the oocytes were allowed to mature in 10% FCS, and the remainder were matured in polyvinyl-alcohol (PVA; 0.3gL−1). For vitrification, oocytes were matured for 22h, partially denuded of cumulus cells, and then vitrified (v-FCS and v-PVA) by the OPS system (Vajta et al. 1988 Mol. Reprod. Dev. 51; 53–58). Fresh untreated controls (c-FCS and c-PVA) were allowed to mature for 24h and immediately fertilized in modified TALP medium with swim-up separated sperm, and cultured. After warming and dilution, vitrified oocytes were cultured in IVM medium for 2h and then fertilized (Day 0). Presumptive zygotes with normal morphology were cultured in SOFaa+amino-acids+myo-inositol+5% FCS (Day 3), and oocytes with a degenerated appearance were counted and discarded. Data were analyzed by ANOVA and Duncan’s test. Results are shown in the Table 1. After warming, we observed severe cryodamage in both v-FCS and v-PVA groups. Rates of degenerated oocytes were 17.8±9.6 and 12.0±9.6 for v-FCS and v-PVA groups, respectively (P>0.05). The presence of PVA instead of FCS did not improve the blastocyst rates obtained from vitrified/warmed oocytes. The use of PVA during IVM (c-PVA) yielded lower (P

Published

2004

32. 94MEIOSIS INHIBITION OF BOVINE OOCYTES: EFFECTS ON SURVIVAL AFTER VITRIFICATION BY OPEN PULLED-STRAW METHOD

Author

L. Fernandez, M. Carbajo, N. Facal, S. de la Varga, C.O. Hidalgo, Enrique J. Gómez, Carmen Díez, and A. Fernandez

Subjects

Embryo culture, Anatomy, Reproductive technology, Biology, Oocyte, Oogenesis, Cryopreservation, Andrology, Endocrinology, medicine.anatomical_structure, Reproductive Medicine, Genetics, medicine, Animal Science and Zoology, Folliculogenesis, Blastocyst, Molecular Biology, Gametogenesis, Developmental Biology, Biotechnology

Abstract

Mammalian oocytes remain one of the most difficult cell types to successfully cryopreserve. The in vitro-maturation protocols (IVM) have a large impact on the oocyte maturation. Consequently, inhibition of meiosis has been used to improve developmental competence of oocytes without reducing blastocyst rates. Moreover, the meiotic stage influences the ability of oocytes to survive cryopreservation. This work analyzes the effect of the inhibition of meiosis (prematuration) on the freezability of the bovine oocyte. Cumulus-oocyte complexes (COCs) were recovered from slaughterhouse ovaries. Inmature oocytes (I) with compact cumulus and evenly granulated cytoplasm were selected. Prematuration (PM) was performed by incubating COCs for 22h in TCM199 NaHCO3 and roscovitine 25μM. IVM was accomplished in TCM199 NaHCO3, 10% FCS, FSH-LH and 17β-estradiol. Oocytes were subjected to 5 treatments prior the vitrification (see table). COCs were partially denuded from cumulus cells and vitrified/warmed using the OPS system (Vajta et al. 1998 Mol. Reprod. Dev. 51, 53–58). Warmed oocytes were fertilized (Day 0) and presumptive zygotes having a normal morphological appearance were cultured in SOFaa+5% of FCS (Day 3); elements with degenerated appearance were discarded and recorded. Fresh oocytes submitted to IVM (c-M) or prematured and matured (c-PM+M) were fertilized and cultured as controls. Data were analyzed by ANOVA and Duncan’s multiple range test and expressed as LSM±SE. Developmental data are referred to the zygotes cultured. Only oocytes vitrified after IVM reached the blastocyst stage, but at lower rates than fresh controls. However, no differences were found between treatments at any developmental stage. Oocytes vitrified both as prematured+matured and immature oocytes showed increased proportions (P

Published

2004

33. Pregnancies and improved early embryonic development with bovine oocytes matured in vitro with 9-cis-retinoic acid

Author

C.O. Hidalgo, N. Facal, P. Duque, Carmen Díez, and Enrique J. Gómez

Subjects

Embryology, Embryogenesis, Morphogenesis, Retinoic acid, Obstetrics and Gynecology, Embryo, Cell Biology, Biology, Oocyte, Embryo transfer, In vitro maturation, Andrology, chemistry.chemical_compound, Endocrinology, medicine.anatomical_structure, Reproductive Medicine, chemistry, embryonic structures, Immunology, medicine, Blastocyst

Abstract

Retinoids have an important role in cell growth, morphogenesis and differentiation. In the present study the developmental potential of bovine oocytes was examined after in vitro maturation in the presence of 9-cis-retinoic acid, a vitamin A metabolite, at 5 nmol l(-1) in chemically defined conditions. Experiments studied early in vitro development, blastocyst differential cell counts and the capacity of embryos to establish pregnancy after transfer to recipients. After in vitro fertilization and culture in simple medium, blastocyst development and hatching rates increased in oocytes matured with 9-cis-retinoic acid. Addition of ethanol (used as a solvent for 9-cis-retinoic acid) resulted in higher cell counts and proportions of cells in the inner mass of day 7 blastocysts. Day 8 blastocysts represented most differences observed in the number of cells. In these embryos, ethanol and 9-cis-retinoic acid increased both the number of cells and proportions in the inner mass. However, while ethanol treatment reduced the number of cells in the trophectoderm, 9-cis-retinoic acid did not. The total number of cells was unaffected by treatment within 1 day, although untreated oocytes lead to day 8 blastocysts with reduced total cell counts. Once transferred to recipients, both fresh and vitrified-warmed blastocysts derived from oocytes matured with 9-cis-retinoic acid yielded more pregnancies at day 60. Modifications of retinoid metabolism affect development and trophectoderm differentiation, and in vitro maturation with 9-cis-retinoic acid increased the developmental competence of the oocyte.