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2. Cooling rate modifies the location of aquaporin 3 in spermatozoa of sheep and goat

Author

Agencia Estatal de Investigación (España), Pequeño, Belén [0000-0003-3962-1982], Millán de la Blanca, María Gemma [0000-0002-2810-8510], Castaño, Cristina [0000-0003-1134-1436], Toledano-Díaz, A. [0000-0001-6679-485X], Esteso, Milagros C. [0000-0002-8963-5736], Arrebola, Francisco A. [0000-0002-5571-7258], Ungerfeld, Rodolfo [0000-0003-4685-2105], Martínez-Madrid, Belén [0000-0001-6852-4597], Álvarez-Rodríguez, Manuel [0000-0003-0120-354X], Rodriguez-Martinez, Heriberto [0000-0002-5194-2124], Santiago Moreno, Julián [0000-0001-5551-8120], Pequeño, Belén, Millán de la Blanca, María Gemma, Castaño, Cristina, Toledano-Díaz, A., Esteso, Milagros C., Alba, Esther, Arrebola, Francisco A., Ungerfeld, Rodolfo, Martínez-Madrid, Belén, Álvarez-Rodríguez, Manuel, Rodriguez-Martinez, Heriberto, Santiago Moreno, Julián, Agencia Estatal de Investigación (España), Pequeño, Belén [0000-0003-3962-1982], Millán de la Blanca, María Gemma [0000-0002-2810-8510], Castaño, Cristina [0000-0003-1134-1436], Toledano-Díaz, A. [0000-0001-6679-485X], Esteso, Milagros C. [0000-0002-8963-5736], Arrebola, Francisco A. [0000-0002-5571-7258], Ungerfeld, Rodolfo [0000-0003-4685-2105], Martínez-Madrid, Belén [0000-0001-6852-4597], Álvarez-Rodríguez, Manuel [0000-0003-0120-354X], Rodriguez-Martinez, Heriberto [0000-0002-5194-2124], Santiago Moreno, Julián [0000-0001-5551-8120], Pequeño, Belén, Millán de la Blanca, María Gemma, Castaño, Cristina, Toledano-Díaz, A., Esteso, Milagros C., Alba, Esther, Arrebola, Francisco A., Ungerfeld, Rodolfo, Martínez-Madrid, Belén, Álvarez-Rodríguez, Manuel, Rodriguez-Martinez, Heriberto, and Santiago Moreno, Julián

Abstract

The freeze-thawing process induces osmotic changes that may affect the membrane domain location of aquaporins’ (AQP) in spermatozoa. Recent studies suggest that changes in AQP3 localization allows better sperm osmo-adaptation, improving the cryoresistance. Ultra-rapid freezing is an alternative cryopreservation technique that requires less equipment than conventional freezing, and it is faster, simpler and can be used in the field. This study aimed to determine the influence of freezing-thawing rates (slow (control) vs. ultra-rapid) on AQP3 expression and location in the spermatozoa from small ruminants (sheep and goats) and its relationship with sperm cryo-damage. Spermatozoa were collected from 10 Merino rams and 10 Murciano-Granadina bucks. The presence and distribution of AQP3 were assessed by Western blotting and immunocytochemistry (ICC), employing a commercial rabbit polyclonal antibody. Sperm motility was CASA system-analyzed, and membrane and acrosome integrity assessed by fluorescence (PI/PNA-FITC). Western blotting did not detect a significant effect of freezing-thawing rate on the amount of AQP3 while ICC found freezing-thawing rate affecting AQP3 location (P<0.05). In both species, the percentages of spermatozoa showing AQP3 in the post-acrosome region, mid-piece, and principal piece of the tail were greater in samples cryopreserved by slow freezing-thawing (control) than ultra-rapid freezing-thawing rates (P<0.05). Spermatozoa cryopreserved using ultra-rapid freezing-thawing showed decrease motility, plasma membrane, and acrosome integrity (P<0.05), which might be related, at least in part, to a lower expression of AQP3. In conclusion, the cooling rate modifies the location of AQP3 in spermatozoa of sheep and goat, which might be associated with sperm cryosurvival.

Published
2024

4. Review: Sperm cryopreservation in wild small ruminants: morphometric, endocrine and molecular basis of cryoresistance

Author

Martínez Madrid, Carmen Belén, Santiago-Moreno, Julián, Toledano-Díaz, Adolfo, Castaño, Cristina, Velázquez, Rosario, Bóveda, Paula, O’Brien, Emma, Peris-Frau, Patricia, Pequeño, Belén, Esteso, Milagros, Martínez Madrid, Carmen Belén, Santiago-Moreno, Julián, Toledano-Díaz, Adolfo, Castaño, Cristina, Velázquez, Rosario, Bóveda, Paula, O’Brien, Emma, Peris-Frau, Patricia, Pequeño, Belén, and Esteso, Milagros

Abstract

Author contributions JSM: Conceptualisation, Writing – review and editing. ATD, CC, RV, PB, PPF, BP, EO, BMM, and MCE: Writing – original draft., Reproductive technologies can help to protect wild ruminant species from becoming extinct. In addition, the decline in some wild game species has also raised interest in reproductive technologies to increase the number of animals that can be produced. Most biobanking efforts have focused on developing effective protocols for preserving sperm, oocytes, and embryos. Cryopreservation of sperm remains the least invasive method and the cheapest procedure for germplasm storage. Over the last few years, several reproductive biotechnologies have been developed beyond the conventional freezing of spermatozoa. These include ultra-rapid freezing techniques. Nevertheless, fertility results after artificial insemination using frozen-thawed spermatozoa are not always acceptable in wild small ruminants. Moreover, these technological efforts have met variable success related to the sample’s origin (epididymal retrieved postmortem or ejaculated) and the season of sperm sample collection and storage. Epididymal sperm shows higher cryoresistance than ejaculated sperm. Changes in sperm proteome between epididymal and ejaculated sperm seem to contribute to this different cryotolerance. The role of endocrine status has been studied in some wild species to better understand the underlying mechanism of the annual variation in ruminant sperm cryoresistance. Seasonal changes in testosterone and prolactin are involved in sperm cryoresistance; sperm recovery and cryopreservation are recommended around the end of the rutting season, when good quality sperm samples can still be obtained, testosterone levels have already decreased, and prolactin concentrations remain low. The mechanisms of hormone action on sperm freezability are not well known. Still, it has been suggested that testosterone affects cell proliferation in the testis, during spermatogenesis, and membrane properties of sperm cells during their transit through the reproductive tract, which might influence their cryotolerance. Recent, Agencia Estatal de Investigación (AEI), Depto. de Medicina y Cirugía Animal, Fac. de Veterinaria, TRUE, pub

Published
2024

5. Location of aquaporins 3, 7 and 10 in frozen-thawed ejaculated and cauda epididymal spermatozoa from the Iberian ibex, mouflon, and chamois

Author

Pequeño, Belén, Martínez Madrid, Carmen Belén, Castaño, Cristina, Toledano-Díaz, Adolfo, Bóveda, Paula, Esteso, Milagros C., Gómez-Guillamón, Félix, Prieto, Paloma, Marcos-Beltrán, Jaime L., Alvarez-Rodriguez, Manuel, Rodriguez-Martinez, Heriberto, Santiago-Moreno, Julián, Pequeño, Belén, Martínez Madrid, Carmen Belén, Castaño, Cristina, Toledano-Díaz, Adolfo, Bóveda, Paula, Esteso, Milagros C., Gómez-Guillamón, Félix, Prieto, Paloma, Marcos-Beltrán, Jaime L., Alvarez-Rodriguez, Manuel, Rodriguez-Martinez, Heriberto, and Santiago-Moreno, Julián

Abstract

Pequeño B was the recipient of a grant for pre-doctoral researchers from AEI (PRE2018–085637)., Spermatozoa collected from the cauda epididymis of wild ruminants are more cryoresistant than ejaculated spermatozoa. Changes in the membrane location of aquaporins (AQPs) follow the osmotic changes that occur during freeze-thawing, and might influence the cryosurvival of spermatozoa depending on their source. This work reports the location of AQP3, AQP7 and AQP10 in the cauda epididymal and post-ejaculation spermatozoa of three wild mountain ungulate species (Iberian ibex, mouflon, and chamois), as determined by Western blotting (WB) and immunocytochemistry (ICC) using commercial rabbit polyclonal primary antibodies. WB confirmed the presence of all three AQPs in the spermatozoa of all the studied species, while ICC showed AQP3 to be mainly located in the sperm acrosome, mid-piece, principal piece, and end piece, both in cauda epididymal and ejaculated cells. The percentage of ejaculated spermatozoa showing AQP3 in the principal piece was higher in the ibex than in the chamois (P < 0.05), and higher in epididymal spermatozoa in the mouflon than in the chamois (P < 0.05). AQP7 was located in the acrosome of both epididymal and ejaculated spermatozoa, as well as in the cytoplasmic droplet of the epididymal spermatozoa of all three species. No differences were seen between the species with respect to the percentage of spermatozoa showing AQP7. AQP10 was located mainly in the mid-piece, principal piece and end piece of the sperm tail in both epididymal and ejaculated spermatozoa. The percentage of mouflon spermatozoa with AQP10 in the end piece was higher in the cauda epididymal than in the ejaculated spermatozoa (P < 0.05). In conclusion, except for AQP10 in the mouflon, the locations of the studied AQPs are similar in epididymal and ejaculated spermatozoa, with inter-species differences seen only for AQP3. Further studies are needed to determine what this might mean with respect to sperm cryopreservation., Agencia Estatal de Investigación (AEI), Ministerio de Ciencia e Innovación, FEDER, Depto. de Medicina y Cirugía Animal, Fac. de Veterinaria, TRUE, pub

Published
2024

6. DNA integrity and viability of testicular cells from diverse wild species after slow freezing or vitrification

Author

Agencia Estatal de Investigación (España), Ministerio de Ciencia e Innovación (España), Fundación Parques Reunidos, CSIC - Instituto Nacional de Investigación y Tecnología Agraria y Alimentaria (INIA), European Commission, Peris-Frau, Patricia [0000-0001-6266-0635], Martínez-Nevado, Eva [0000-0002-8994-4205], Toledano Díaz, Adolfo [0000-0001-6679-485X], Pequeño, Belén [0000-0003-3962-1982], Martínez-Madrid, Belén [0000-0001-6852-4597], Esteso, Milagros C. [0000-0002-8963-5736], Santiago Moreno, Julián [0000-0001-5551-8120], Peris-Frau, Patricia, Benito-Blanco, Julia, Martínez-Nevado, Eva, Toledano-Díaz, A., Castaño, Cristina, Velázquez, Rosario, Pequeño, Belén, Martínez-Madrid, Belén, Esteso, Milagros C., Santiago Moreno, Julián, Agencia Estatal de Investigación (España), Ministerio de Ciencia e Innovación (España), Fundación Parques Reunidos, CSIC - Instituto Nacional de Investigación y Tecnología Agraria y Alimentaria (INIA), European Commission, Peris-Frau, Patricia [0000-0001-6266-0635], Martínez-Nevado, Eva [0000-0002-8994-4205], Toledano Díaz, Adolfo [0000-0001-6679-485X], Pequeño, Belén [0000-0003-3962-1982], Martínez-Madrid, Belén [0000-0001-6852-4597], Esteso, Milagros C. [0000-0002-8963-5736], Santiago Moreno, Julián [0000-0001-5551-8120], Peris-Frau, Patricia, Benito-Blanco, Julia, Martínez-Nevado, Eva, Toledano-Díaz, A., Castaño, Cristina, Velázquez, Rosario, Pequeño, Belén, Martínez-Madrid, Belén, Esteso, Milagros C., and Santiago Moreno, Julián

Abstract

Cryopreservation of testicular tissues offers new possibilities to protect endangered species, genetically valuable individuals or even the fertility potential of prepubertal individuals who have died unexpectedly. However, the use of this technique still remains a challenge. In this study, slow freezing and vitrification of testicular tissue was investigated to find out which cryopreservation method could better preserve the viability and DNA integrity of testicular germ cells in diverse wild species.

Published
2023

7. Location of aquaporins 3, 7 and 10 in frozen-thawed ejaculated and cauda epididymal spermatozoa from the Iberian ibex, mouflon, and chamois

Author

Agencia Estatal de Investigación (España), European Commission, Ministerio de Ciencia e Innovación (España), Pequeño, Belén [0000-0003-3962-1982], Martínez-Madrid, Belén [0000-0001-6852-4597], Castaño, Cristina [0000-0003-1134-1436], Toledano-Díaz, A. [0000-0001-6679-485X], Bóveda, Paula [0000-0001-5749-4345], Esteso, Milagros C. [0000-0002-8963-5736], Gómez-Guillamón, Félix [0000-0001-9757-9589], Álvarez-Rodríguez, Manuel [0000-0003-0120-354X], Rodriguez-Martinez, Heriberto [0000-0002-5194-2124], Santiago Moreno, Julián [0000-0001-5551-8120], Pequeño, Belén, Martínez-Madrid, Belén, Castaño, Cristina, Toledano-Díaz, A., Bóveda, Paula, Esteso, Milagros C., Gómez-Guillamón, Félix, Prieto, Paloma, Marcos-Beltrán, J. L., Álvarez-Rodríguez, Manuel, Rodriguez-Martinez, Heriberto, Santiago Moreno, Julián, Agencia Estatal de Investigación (España), European Commission, Ministerio de Ciencia e Innovación (España), Pequeño, Belén [0000-0003-3962-1982], Martínez-Madrid, Belén [0000-0001-6852-4597], Castaño, Cristina [0000-0003-1134-1436], Toledano-Díaz, A. [0000-0001-6679-485X], Bóveda, Paula [0000-0001-5749-4345], Esteso, Milagros C. [0000-0002-8963-5736], Gómez-Guillamón, Félix [0000-0001-9757-9589], Álvarez-Rodríguez, Manuel [0000-0003-0120-354X], Rodriguez-Martinez, Heriberto [0000-0002-5194-2124], Santiago Moreno, Julián [0000-0001-5551-8120], Pequeño, Belén, Martínez-Madrid, Belén, Castaño, Cristina, Toledano-Díaz, A., Bóveda, Paula, Esteso, Milagros C., Gómez-Guillamón, Félix, Prieto, Paloma, Marcos-Beltrán, J. L., Álvarez-Rodríguez, Manuel, Rodriguez-Martinez, Heriberto, and Santiago Moreno, Julián

Abstract

Spermatozoa collected from the cauda epididymis of wild ruminants are more cryoresistant than ejaculated spermatozoa. Changes in the membrane location of aquaporins (AQPs) follow the osmotic changes that occur during freeze-thawing, and might influence the cryosurvival of spermatozoa depending on their source. This work reports the location of AQP3, AQP7 and AQP10 in the cauda epididymal and post-ejaculation spermatozoa of three wild mountain ungulate species (Iberian ibex, mouflon, and chamois), as determined by Western blotting (WB) and immunocytochemistry (ICC) using commercial rabbit polyclonal primary antibodies. WB confirmed the presence of all three AQPs in the spermatozoa of all the studied species, while ICC showed AQP3 to be mainly located in the sperm acrosome, mid-piece, principal piece, and end piece, both in cauda epididymal and ejaculated cells. The percentage of ejaculated spermatozoa showing AQP3 in the principal piece was higher in the ibex than in the chamois (P < 0.05), and higher in epididymal spermatozoa in the mouflon than in the chamois (P < 0.05). AQP7 was located in the acrosome of both epididymal and ejaculated spermatozoa, as well as in the cytoplasmic droplet of the epididymal spermatozoa of all three species. No differences were seen between the species with respect to the percentage of spermatozoa showing AQP7. AQP10 was located mainly in the mid-piece, principal piece and end piece of the sperm tail in both epididymal and ejaculated spermatozoa. The percentage of mouflon spermatozoa with AQP10 in the end piece was higher in the cauda epididymal than in the ejaculated spermatozoa (P < 0.05). In conclusion, except for AQP10 in the mouflon, the locations of the studied AQPs are similar in epididymal and ejaculated spermatozoa, with inter-species differences seen only for AQP3. Further studies are needed to determine what this might mean with respect to sperm cryopreservation.

Published
2023

8. Review: Sperm cryopreservation in wild small ruminants: morphometric, endocrine and molecular basis of cryoresistance

Author

Agencia Estatal de Investigación (España), Santiago Moreno, Julián [0000-0001-5551-8120], Toledano-Diaz, A. [0000-0001-6679-485X], Castaño, Cristina [0000-0003-1134-1436], Velázquez, Rosario [0009-0009-2115-4715], Bóveda, Paula [0000-0001-5749-4345], Peris-Frau, Patricia [0000-0001-6266-0635], Pequeño, Belén [0000-0003-3962-1982], Martínez-Madrid, Belén [0000-0001-6852-4597], Esteso, Milagros C. [0000-0002-8963-5736], Santiago Moreno, Julián, Toledano-Díaz, A., Castaño, Cristina, Velázquez, Rosario, Bóveda, Paula, O'Brien, Emma, Peris-Frau, Patricia, Pequeño, Belén, Martínez-Madrid, Belén, Esteso, Milagros C., Agencia Estatal de Investigación (España), Santiago Moreno, Julián [0000-0001-5551-8120], Toledano-Diaz, A. [0000-0001-6679-485X], Castaño, Cristina [0000-0003-1134-1436], Velázquez, Rosario [0009-0009-2115-4715], Bóveda, Paula [0000-0001-5749-4345], Peris-Frau, Patricia [0000-0001-6266-0635], Pequeño, Belén [0000-0003-3962-1982], Martínez-Madrid, Belén [0000-0001-6852-4597], Esteso, Milagros C. [0000-0002-8963-5736], Santiago Moreno, Julián, Toledano-Díaz, A., Castaño, Cristina, Velázquez, Rosario, Bóveda, Paula, O'Brien, Emma, Peris-Frau, Patricia, Pequeño, Belén, Martínez-Madrid, Belén, and Esteso, Milagros C.

Abstract

Reproductive technologies can help to protect wild ruminant species from becoming extinct. In addition, the decline in some wild game species has also raised interest in reproductive technologies to increase the number of animals that can be produced. Most biobanking efforts have focused on developing effective protocols for preserving sperm, oocytes, and embryos. Cryopreservation of sperm remains the least invasive method and the cheapest procedure for germplasm storage. Over the last few years, several reproductive biotechnologies have been developed beyond the conventional freezing of spermatozoa. These include ultra-rapid freezing techniques. Nevertheless, fertility results after artificial insemination using frozen-thawed spermatozoa are not always acceptable in wild small ruminants. Moreover, these technological efforts have met variable success related to the sample's origin (epididymal retrieved postmortem or ejaculated) and the season of sperm sample collection and storage. Epididymal sperm shows higher cryoresistance than ejaculated sperm. Changes in sperm proteome between epididymal and ejaculated sperm seem to contribute to this different cryotolerance. The role of endocrine status has been studied in some wild species to better understand the underlying mechanism of the annual variation in ruminant sperm cryoresistance. Seasonal changes in testosterone and prolactin are involved in sperm cryoresistance; sperm recovery and cryopreservation are recommended around the end of the rutting season, when good quality sperm samples can still be obtained, testosterone levels have already decreased, and prolactin concentrations remain low. The mechanisms of hormone action on sperm freezability are not well known. Still, it has been suggested that testosterone affects cell proliferation in the testis, during spermatogenesis, and membrane properties of sperm cells during their transit through the reproductive tract, which might influence their cryotolerance. Recent

Published
2023

9. Influence of Prolactin Secretion Changes on Sperm Head Size and Freezability in Ibex and Mouflon

Author

Bóveda Gómez, P. [0000-0001-5749-4345], Martínez-Fresneda, Lucía [0000-0002-0967-8593], Toledano Díaz, Adolfo [0000-0001-6679-485X], Esteso, Milagros C. [0000-0002-8963-5736], Ungerfeld, Rodolfo [0000-0003-4685-2105], López Sebastián, Antonio [0000-0001-8695-7441], Santiago Moreno, Julián [0000-0001-5551-8120], Velázquez, Rosario, Bóveda, Paula, Martínez-Fresneda, Lucía, Mejía, Octavio, Oteo, M., Toledano-Díaz, A., Castaño, Cristina, Esteso, Milagros C., Ungerfeld, Rodolfo, López Sebastián, Antonio, Santiago Moreno, Julián, Bóveda Gómez, P. [0000-0001-5749-4345], Martínez-Fresneda, Lucía [0000-0002-0967-8593], Toledano Díaz, Adolfo [0000-0001-6679-485X], Esteso, Milagros C. [0000-0002-8963-5736], Ungerfeld, Rodolfo [0000-0003-4685-2105], López Sebastián, Antonio [0000-0001-8695-7441], Santiago Moreno, Julián [0000-0001-5551-8120], Velázquez, Rosario, Bóveda, Paula, Martínez-Fresneda, Lucía, Mejía, Octavio, Oteo, M., Toledano-Díaz, A., Castaño, Cristina, Esteso, Milagros C., Ungerfeld, Rodolfo, López Sebastián, Antonio, and Santiago Moreno, Julián

Abstract

Aim: This work examined the influence of induced changes in prolactin (PRL) secretion on sperm cryoresistance of ibex and the mouflon. Materials and Methods: PRL secretion was modified in a first experiment by the use of bromocriptine (BCR, dopamine agonist) during the non-breeding season, and in a second experiment by the use of sulpiride (SLP, dopamine D2-receptor antagonist) during the rutting season. Slow and ultra-rapid freezing protocols were used to cryopreserve sperm samples. Results: BCR decreased blood plasma PRL concentrations, whereas SLP increased them. Cryoresistance ratios (CRs) for curvilinear velocity (VCL), straight-line velocity (VSL), and average path velocity (VAP) in BCR-treated mouflons were lower than in controls using slow-freezing (p < 0.05), while CRs of motility and morphologically normal sperm of BCR-treated mouflons were greater than controls with ultra-rapid freezing (p < 0.05). BCR increased the head sperm dimensions in ibexes (p < 0.001); conversely, BCR decreased the head dimensions in mouflons (p < 0.001). CR-motility, CR-amplitude of lateral head displacement (ALH), CR-viability, and CR-acrosome integrity in SLP-treated mouflons were lower than in controls with slow-freezing (p < 0.01); CR-viability and CR-acrosome were lower than controls with ultra-rapid freezing (p < 0.05). In ibexes, CR-ALH was lower for SLP-treated (p < 0.05). SLP treatment increased head dimensions in ibexes (p < 0.001) but did not affect the sperm head of mouflons. Conclusion: Our findings show that high levels of blood plasma PRL negatively affect the cryoresistance of ibex and mouflon sperm.

Published
2022

10. Cryopreservation of testicular tissue from the dog (Canis familiaris) and wild boar (Sus scrofa) by slow freezing and vitrification: Differences in cryoresistance according to cell type

Author

Agencia Estatal de Investigación (España), Comunidad de Madrid, Centro de Recuperación de Animales Silvestres (España), Centro Veterinario Aluche-Las Águilas, Castaño, C. [0000-0003-1134-1436], Bóveda, P. [0000-0001-5749-4345], Toledano Díaz, Adolfo [0000-0001-6679-485X], Esteso, Milagros C. [0000-0002-8963-5736], Gadea, J. [0000-0002-3474-7626], Villaverde-Morcillo, S. [0000-0002-4879-6007], Santiago Moreno, Julián [0000-0001-5551-8120], Picazo, C M., Castaño, Cristina, Bóveda, Paula, Toledano-Díaz, A., Velázquez, Rosario, Pequeño, Belén, Esteso, Milagros C., Gadea, J., Villaverde-Morcillo, S., Cerdeira, J., Santiago Moreno, Julián, Agencia Estatal de Investigación (España), Comunidad de Madrid, Centro de Recuperación de Animales Silvestres (España), Centro Veterinario Aluche-Las Águilas, Castaño, C. [0000-0003-1134-1436], Bóveda, P. [0000-0001-5749-4345], Toledano Díaz, Adolfo [0000-0001-6679-485X], Esteso, Milagros C. [0000-0002-8963-5736], Gadea, J. [0000-0002-3474-7626], Villaverde-Morcillo, S. [0000-0002-4879-6007], Santiago Moreno, Julián [0000-0001-5551-8120], Picazo, C M., Castaño, Cristina, Bóveda, Paula, Toledano-Díaz, A., Velázquez, Rosario, Pequeño, Belén, Esteso, Milagros C., Gadea, J., Villaverde-Morcillo, S., Cerdeira, J., and Santiago Moreno, Julián

Abstract

Sperm cryopreservation is the most common procedure used to establish germplasm banks for endangered species - but sometimes sperm cells cannot be obtained. In such cases, freezing testicular tissue may be the only option. The testes contains germ cells at different stages of differentiation, including spermatogonia, primary spermatocytes, secondary spermatocytes, spermatids, and spermatozoa, among which differences in cryoresistance might be expected. The present work compares the viability and DNA integrity of 'rounded' cells, and of elongated spermatids and spermatozoa, from the dog and wild boar, following the cryopreservation of testicular tissue by slow freezing or vitrification. Cell viability was analyzed by PI/SYBR14 staining, and DNA integrity via the TUNEL technique. For wild boar, no significant differences were seen between the two methods with respect to the percentage of viable cells, nor in the percentage of cells with DNA damage. In the dog, the percentage of viable rounded germ cells (65.0 ± 2.4%) was higher (P < 0.05) after vitrification than after slow freezing (45.1 ± 6.7%). No difference was found between the two methods in terms of the viability of elongated cells. For rounded cells, the percentage of intact DNA was greater (P < 0.05) after vitrification (90.5 ± 2.1%) than after slow freezing (42.6 ± 11.0%), while for elongated spermatids and spermatozoa it was higher (P < 0.05) after slow freezing (66.9 ± 6.1%) than after vitrification (50.7 ± 4.5%). Thus, the response to cryopreservation is cell type-, cryopreservation type-, and species-dependent. Vitrification would appear to be the most appropriate method for preserving dog testicular tissue given the associated high cell viability and low degree of DNA fragmentation, while in wild boar, either method might be used.

Published
2022

11. Birchen and Blue Leonesa sperm cryopreservation: a new technique for evaluating the integrity of cockerel sperm membranes

Author

European Commission, Castaño, Cristina [0000-0003-1134-1436], Bernal, B [0000-0001-9144-1554], Esteso, Milagros C. [0000-0002-8963-5736], Toledano Díaz, Adolfo [0000-0001-6679-485X], Blesbois, E [0000-0001-8182-6602], Santiago Moreno, Julián [0000-0001-5551-8120], López Sebastián, Antonio [0000-0001-8695-7441], García-Gil, María [0000-0003-2856-277X], Bernal Juárez, Berenice, Castaño, Cristina, Esteso, Milagros C., Toledano-Díaz, A., Domínguez-González, Miguel A., García-Gil, María, López Sebastián, Antonio, Campo, J. L., Blesbois, E., Santiago Moreno, Julián, European Commission, Castaño, Cristina [0000-0003-1134-1436], Bernal, B [0000-0001-9144-1554], Esteso, Milagros C. [0000-0002-8963-5736], Toledano Díaz, Adolfo [0000-0001-6679-485X], Blesbois, E [0000-0001-8182-6602], Santiago Moreno, Julián [0000-0001-5551-8120], López Sebastián, Antonio [0000-0001-8695-7441], García-Gil, María [0000-0003-2856-277X], Bernal Juárez, Berenice, Castaño, Cristina, Esteso, Milagros C., Toledano-Díaz, A., Domínguez-González, Miguel A., García-Gil, María, López Sebastián, Antonio, Campo, J. L., Blesbois, E., and Santiago Moreno, Julián

Abstract

1. Birchen and Blue Leonesa are two endangered chicken breeds mainly raised in Curueño Valley in North Spain. The establishment of a germplasm bank to guarantee the preservation of these breeds is needed. However, cockerels from different breeder flocks can show variance in semen cryoresistance.2. The following work focused on the sperm characterisation and cryopreservation of Birchen and Blue Leonesa cockerels from four different breeders. A total of 30 semen pools were analysed. Besides conventional sperm analysis, including motility by computer-aided sperm analysis (CASA) and DNA fragmentation by TUNEL, the present study tested a double staining method (MitoTrackerTM Green FM/propidium iodide). This gave simultaneous assessment of plasma and acrosomal and mitochondrial membranes, which were previously validated by SYBR-14/PI, CASA, aniline blue and TUNEL.3. No significant differences were found among fresh semen variables between breeds and breeders. For post-thawed variables, significant differences (P < 0.05) were found between breeders in sperm viability (58.0 ± 1.90 breeder D vs. 35.2 ± 7.41 breeder A, 37.2 ± 4.09 breeder B and 22.3 ± 5.92 breeder C) and DNA fragmentation (62.4 ± 9.91 breeder C vs. 31.8 ± 7.08 breeder B and 24.5 ± 5.49 breeder D). The lowest DNA fragmentation values for semen from breeder D birds were coincident with higher integrity of the mitochondrial membrane.4. The results revealed higher sperm cryoresistance in the cockerels from one of the breeders, possibly due to differences in management system (e.g. diet, housing, control of stress elements and pathogens, reproduction practices or maintenance of genetic diversity). These differences may determine the sperm freezability, and thus the effectiveness of developing a germplasm bank., r

Published
2022

12. Use of native chicken breeds (Gallus gallus domesticus) for the development of suitable methods of Cantabrian capercaillie (Tetrao urogallus cantabricus) semen cryopreservation

Author

Fundación Biodiversidad, Ministerio para la Transición Ecológica y el Reto Demográfico (España), Castaño, Cristina [0000-0003-1134-1436], Toledano Díaz, Adolfo [0000-0001-6679-485X], Caamaño, José Néstor [0000-0001-6449-5784], Fidalgo, Luis Eusebio [0000-0001-9184-0942], Esteso, Milagros C. [0000-0002-8963-5736], García-Casado, Pedro [0000-0002-1242-1035], Lukaszewicz, Ewa [0000-0002-9505-0056], Santiago Moreno, Julián [0000-0001-5551-8120], Hidalgo, Carlos Olegario [0000-0002-9810-1517], O'Brien, Emma, Castaño, Cristina, Toledano-Díaz, A., Caamaño, J. N., Hidalgo, Carlos Olegario, Fidalgo, Luis Eusebio, López-Beceiro, Ana, Esteso, Milagros C., Balsera, Ramón, García-Casado, Pedro, Lukaszewicz, Ewa, Santiago Moreno, Julián, Fundación Biodiversidad, Ministerio para la Transición Ecológica y el Reto Demográfico (España), Castaño, Cristina [0000-0003-1134-1436], Toledano Díaz, Adolfo [0000-0001-6679-485X], Caamaño, José Néstor [0000-0001-6449-5784], Fidalgo, Luis Eusebio [0000-0001-9184-0942], Esteso, Milagros C. [0000-0002-8963-5736], García-Casado, Pedro [0000-0002-1242-1035], Lukaszewicz, Ewa [0000-0002-9505-0056], Santiago Moreno, Julián [0000-0001-5551-8120], Hidalgo, Carlos Olegario [0000-0002-9810-1517], O'Brien, Emma, Castaño, Cristina, Toledano-Díaz, A., Caamaño, J. N., Hidalgo, Carlos Olegario, Fidalgo, Luis Eusebio, López-Beceiro, Ana, Esteso, Milagros C., Balsera, Ramón, García-Casado, Pedro, Lukaszewicz, Ewa, and Santiago Moreno, Julián

Abstract

The Cantabrian capercaillie (Tetrao urogallus cantabricus) is critically endangered. This subspecies has the lowest genetic variability and it is in regression. It belongs to Phasianidae family; therefore, the domestic chicken (Gallus gallus domesticus) could be a good model for developing reproductive technologies for use in capercaillie populations with low availability of animals.

Published
2022

13. DNA integrity and viability of testicular cells from diverse wild species after slow freezing or vitrification

Author

Peris-Frau, Patricia, primary, Benito-Blanco, Julia, additional, Martínez-Nevado, Eva, additional, Toledano-Díaz, Adolfo, additional, Castaño, Cristina, additional, Velázquez, Rosario, additional, Pequeño, Belén, additional, Martinez-Madrid, Belén, additional, Esteso, Milagros C., additional, and Santiago-Moreno, Julián, additional

Published
2023
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15. Influence of circulating testosterone concentration on sperm cryoresistance: The ibex as an experimental model

Author

Ministerio de Ciencia e Innovación (España), European Commission, Agencia Estatal de Investigación (España), Ministerio de Economía y Competitividad (España), Universidad Nacional Autónoma de México, Bóveda, Paula [0000-0001-5749-4345], Esteso, Milagros C. [0000-0002-8963-5736], Castaño, Cristina [0000-0003-1134-1436], Toledano-Díaz, Adolfo [0000-0001-6679-485X], López Sebastián, Antonio [0000-0001-8695-7441], Millán de la Blanca, María Gemma [0000-0002-2810-8510], Ungerfeld, Rodolfo [0000-0003-4685-2105], Santiago Moreno, Julián [0000-0001-5551-8120], Bóveda, Paula, Esteso, Milagros C., Velázquez, Rosario, Castaño, Cristina, Toledano-Díaz, A., López Sebastián, Antonio, Mejía, Octavio, Millán de la Blanca, María Gemma, Ungerfeld, Rodolfo, Santiago Moreno, Julián, Ministerio de Ciencia e Innovación (España), European Commission, Agencia Estatal de Investigación (España), Ministerio de Economía y Competitividad (España), Universidad Nacional Autónoma de México, Bóveda, Paula [0000-0001-5749-4345], Esteso, Milagros C. [0000-0002-8963-5736], Castaño, Cristina [0000-0003-1134-1436], Toledano-Díaz, Adolfo [0000-0001-6679-485X], López Sebastián, Antonio [0000-0001-8695-7441], Millán de la Blanca, María Gemma [0000-0002-2810-8510], Ungerfeld, Rodolfo [0000-0003-4685-2105], Santiago Moreno, Julián [0000-0001-5551-8120], Bóveda, Paula, Esteso, Milagros C., Velázquez, Rosario, Castaño, Cristina, Toledano-Díaz, A., López Sebastián, Antonio, Mejía, Octavio, Millán de la Blanca, María Gemma, Ungerfeld, Rodolfo, and Santiago Moreno, Julián

Abstract

Recent studies have noted that the circulating testosterone concentration may affect the ability of spermatozoa to survive cryopreservation. However, few attempts to confirm such a relationship have been made. Wild ruminant species have very marked seasonal changes in their reproductive function and strong annual changes in their plasma testosterone concentration.

Published
2021

16. Cryopreservation of ferret (Mustela putorius furo) sperm collected by rectal massage and electroejaculation: Comparison of a decelerating and an accelerating freezing rate protocol

Author

Fundación Biodiversidad, Ministerio para la Transición Ecológica y el Reto Demográfico (España), Toledano Díaz, Adolfo [0000-0001-6679-485X], Castaño, Cristina [0000-0003-1134-1436], Bóveda, Paula [0000-0001-5749-4345], López Sebastián, Antonio [0000-0001-8695-7441], Martínez-Nevado, Eva [0000-0002-8994-4205], Villaverde-Morcillo, S. [0000-0002-4879-6007], Esteso, Milagros C. [0000-0002-8963-5736], Santiago Moreno, Julián [0000-0001-5551-8120], Toledano-Díaz, A., Castaño, Cristina, Velázquez, Rosario, Bóveda, Paula, López Sebastián, Antonio, Martínez-Nevado, Eva, Villaverde-Morcillo, S., Esteso, Milagros C., Santiago Moreno, Julián, Fundación Biodiversidad, Ministerio para la Transición Ecológica y el Reto Demográfico (España), Toledano Díaz, Adolfo [0000-0001-6679-485X], Castaño, Cristina [0000-0003-1134-1436], Bóveda, Paula [0000-0001-5749-4345], López Sebastián, Antonio [0000-0001-8695-7441], Martínez-Nevado, Eva [0000-0002-8994-4205], Villaverde-Morcillo, S. [0000-0002-4879-6007], Esteso, Milagros C. [0000-0002-8963-5736], Santiago Moreno, Julián [0000-0001-5551-8120], Toledano-Díaz, A., Castaño, Cristina, Velázquez, Rosario, Bóveda, Paula, López Sebastián, Antonio, Martínez-Nevado, Eva, Villaverde-Morcillo, S., Esteso, Milagros C., and Santiago Moreno, Julián

Abstract

The domestic ferret (Mustela putorius furo) provides a good model for developing new reproductive technologies for use with threatened related species. Such technologies could also be used in the reproductive management of this pet species. The present work reports an improved freezing protocol for ferret sperm. Semen was collected by electroejaculation plus rectal massage (in an attempt to reduce the electrical stimulation necessary) from five adult male ferrets, and then subjected to one of two freezing protocols: (a) from 5 to -35°C at 40°C/min, then from -35 to -65°C at 17°C/min, and finally from -65 to -85°C at 3°C/min-a decelerating freezing rate; and (b) from 5 to - 10°C at 5°C/min, and then from -10 to -130°C at 60°C/min-an accelerating freezing rate. After thawing, the viability and acrosomal integrity of the sperm frozen via the two-step accelerating method were better than those frozen via the three-step decelerating method (43.3 ± 3.5% and 71.2 ± 3.4% compared with 29.7 ± 3.7% and 58.8 ± 3.4% respectively; p < .05). No differences were seen between the methods with respect to sperm motility variables; most sperm (>90%) remained static with both freezing methods. In conclusion, although the method with accelerating freezing rate was associated with better post-thaw sperm viability and acrosome integrity values, neither of the two freezing methods tested provided adequate motility results after thawing. Combining rectal massage with electrical stimuli seemed to reduce the number of the latter required for successful sperm collection.

Published
2021

17. Sperm Cryopreservation in American Flamingo (Phoenicopterus Ruber): Influence of Cryoprotectants and Seminal Plasma Removal

Author

Fundación Parques Reunidos, CSIC - Instituto Nacional de Investigación y Tecnología Agraria y Alimentaria (INIA), Millán de la Blanca, María Gemma [0000-0002-2810-8510], Martínez-Nevado, Eva [0000-0002-8994-4205], Castaño, Cristina [0000-0003-1134-1436], Bernal, Berenice [0000-0001-9144-1554], Toledano Díaz, Adolfo [0000-0001-6679-485X], Esteso, Milagros C. [0000-0002-8963-5736], Bóveda, Paula [0000-0001-5749-4345], Martínez-Fresneda, Lucía [0000-0002-0967-8593], López Sebastián, Antonio [0000-0001-8695-7441], Santiago Moreno, Julián [0000-0001-5551-8120], Millán de la Blanca, María Gemma, Martínez-Nevado, Eva, Castaño, Cristina, García, Juncal, Bernal Juárez, Berenice, Toledano-Díaz, A., Esteso, Milagros C., Bóveda, Paula, Martínez-Fresneda, Lucía, López Sebastián, Antonio, Santiago Moreno, Julián, Fundación Parques Reunidos, CSIC - Instituto Nacional de Investigación y Tecnología Agraria y Alimentaria (INIA), Millán de la Blanca, María Gemma [0000-0002-2810-8510], Martínez-Nevado, Eva [0000-0002-8994-4205], Castaño, Cristina [0000-0003-1134-1436], Bernal, Berenice [0000-0001-9144-1554], Toledano Díaz, Adolfo [0000-0001-6679-485X], Esteso, Milagros C. [0000-0002-8963-5736], Bóveda, Paula [0000-0001-5749-4345], Martínez-Fresneda, Lucía [0000-0002-0967-8593], López Sebastián, Antonio [0000-0001-8695-7441], Santiago Moreno, Julián [0000-0001-5551-8120], Millán de la Blanca, María Gemma, Martínez-Nevado, Eva, Castaño, Cristina, García, Juncal, Bernal Juárez, Berenice, Toledano-Díaz, A., Esteso, Milagros C., Bóveda, Paula, Martínez-Fresneda, Lucía, López Sebastián, Antonio, and Santiago Moreno, Julián

Abstract

The American flamingo is a useful model for the development of successful semen cryopreservation procedures to be applied to threatened related species from the family Phoenicopteridae, and to permit genetic material banking. Current study sought to develop effective sperm cryopreservation protocols through examining the influences of two permeating cryoprotectants and the seminal plasma removal. During two consecutive years (April), semen samples were collected and frozen from American flamingos. In the first year, the effect of two permeating cryoprotectants, DMA (dimethylacetamide) (6%) or Me2SO (dimethylsulphoxide) (8%), on frozen-thawed sperm variables were compared in 21 males. No differences were seen between DMA and Me2SO for sperm motility, sperm viability, and DNA fragmentation after thawing. In the second year, the role of seminal plasma on sperm cryoresistance was investigated in 31 flamingos. Sperm samples were cryopreserved with and without seminal plasma, using Me2SO (8%) as a cryoprotectant. The results showed that samples with seminal plasma had higher values than samples without seminal plasma for the following sperm variables: Straight line velocity (22.40 µm/s vs. 16.64 µm/s), wobble (75.83% vs. 69.40%), (p < 0.05), linearity (62.73% vs. 52.01%) and straightness (82.38% vs. 73.79%) (p < 0.01); but acrosome integrity was lower (55.56% vs. 66.88%) (p < 0.05). The cryoresistance ratio (CR) was greater in samples frozen with seminal plasma than without seminal plasma for CR-progressive motility (138.72 vs. 54.59), CR-curvilinear velocity (105.98 vs. 89.32), CR-straight line velocity (152.77 vs. 112.58), CR-average path velocity (122.48 vs. 98.12), CR-wobble (111.75 vs. 102.04) (p < 0.05), CR-linearity (139.41 vs. 113.18), and CR-straightness (124.02 vs. 109.97) (p < 0.01). This research demonstrated that there were not differences between Me2SO and DMA to successful freezing sperm of flamingos; seminal plasma removal did not provide a benefit for spe

Published
2021

18. Influence of Prolactin Secretion Changes on Sperm Head Size and Freezability in Ibex and Mouflon

Author

Bóveda Gómez, Paula, primary, Velázquez, Rosario, additional, Martínez-Fresneda, Lucía, additional, Mejía, Octavio, additional, Oteo, Marta, additional, Toledano-Díaz, Adolfo, additional, Castaño, Cristina, additional, Esteso, Milagros Cristina, additional, Ungerfeld, Rodolfo, additional, López-Sebastián, Antonio, additional, and Santiago-Moreno, Julian, additional

Published
2022
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19. Ultra-rapid cooling of ibex sperm by spheres method does not induce a vitreous extracellular state and increases the membrane damages

Author

Agencia Estatal de Investigación (España), Ministerio de Economía y Competitividad (España), European Commission, Bóveda, Paula [0000-0001-5749-4345], Toledano-Diaz, A. [0000-0001-6679-485X], Castaño, Cristina [0000-0003-1134-1436], Esteso, Milagros C. [0000-0002-8963-5736], López Sebastián, Antonio [0000-0001-8695-7441], Rizos, Dimitrios [0000-0001-6813-3940], Bielli, Alejandro [0000-0003-1193-3829], Ungerfeld, Rodolfo [0000-0003-4685-2105], Santiago Moreno, Julián [0000-0001-5551-8120], Bóveda, Paula, Toledano-Díaz, A., Castaño, Cristina, Esteso, Milagros C., López Sebastián, Antonio, Rizos, Dimitrios, Bielli, Alejandro, Ungerfeld, Rodolfo, Santiago Moreno, Julián, Agencia Estatal de Investigación (España), Ministerio de Economía y Competitividad (España), European Commission, Bóveda, Paula [0000-0001-5749-4345], Toledano-Diaz, A. [0000-0001-6679-485X], Castaño, Cristina [0000-0003-1134-1436], Esteso, Milagros C. [0000-0002-8963-5736], López Sebastián, Antonio [0000-0001-8695-7441], Rizos, Dimitrios [0000-0001-6813-3940], Bielli, Alejandro [0000-0003-1193-3829], Ungerfeld, Rodolfo [0000-0003-4685-2105], Santiago Moreno, Julián [0000-0001-5551-8120], Bóveda, Paula, Toledano-Díaz, A., Castaño, Cristina, Esteso, Milagros C., López Sebastián, Antonio, Rizos, Dimitrios, Bielli, Alejandro, Ungerfeld, Rodolfo, and Santiago Moreno, Julián

Abstract

Sperm cryopreservation by ultra-rapid cooling based on dropping small volumes of sperm suspension directly into liquid nitrogen, has been successful in some wild ruminant species, including the Iberian ibex (Capra pyrenaica). In ultra-rapid cooling, the contents of these droplets are expected to enter a stable, glass-like state, but to the best of our knowledge no information exists regarding the presence or absence of ice formation in the extracellular milieu when using this technique. Different modifications to the extracellular milieu likely inflict different types of damage on the plasmalemma, the acrosome and mitochondrial membranes. The aims of the present work were: 1) to examine the physical state of the extracellular milieu after cryopreservation at slow and ultra-rapid cooling rates-and thus determine whether ultra-rapid cooling vitrifies the extracellular milieu; and 2) to compare, using conventional sperm analysis techniques and scanning and transmission electron microscopy, the damage to sperm caused by these two methods. Sperm samples were obtained by the transrectal ultrasound-guided massage method (TUMASG) from anesthetized Iberian ibexes, and cryopreserved using slow and ultra-rapid cooling techniques. Sperm motility (22.95 ± 3.22% vs 4.42 ± 0.86%), viability (25.64 ± 3.71% vs 12.8 ± 2.50%), acrosome integrity (41.45± 3.73% vs 27.00 ± 1.84%) and mitochondrial membrane integrity (16.52 ± 3.75% vs 4.00 ± 0.65%) were better after slow cooling (P<0.001) than after ultra-rapid technique. Cryo-scanning electron microscopy (Cryo-SEM) suggested that the vitrified state was not achieved by ultra-rapid cooling, and that the ice crystals formed were smaller and had more stretchmarks (P<0.001) than after slow cooling. Scanning electron microscopy revealed no differences in the types of damage caused by the examined techniques, although transmission electron microscopy showed the damage to the plasmalemma and mitochondrial membrane to be worse after ultra-rapid

Published
2020

20. Unilateral single vaginal ectopic ureter with ipsilateral hypoplastic and degenerated kidney associated with infertility in iberian ibex (Capra Pyrenaica) does

Author

CSIC - Instituto Nacional de Investigación y Tecnología Agraria y Alimentaria (INIA), Galarza, Diego Andres [0000-0002-0266-5431], Bóveda, Paula [0000-0001-5749-4345], Toledano-Diaz, A. [0000-0001-6679-485X], Castaño, Cristina [0000-0003-1134-1436], Esteso, Milagros C. [0000-0002-8963-5736], López Sebastián, Antonio [0000-0001-8695-7441], Sánchez-Calabuig, M. J. [0000-0002-4280-992X], Santiago Moreno, Julián [0000-0001-5551-8120], Galarza, Diego Andres, Bóveda, Paula, Toledano-Díaz, A., Castaño, Cristina, Esteso, Milagros C., López Sebastián, Antonio, Sánchez-Calabuig, M. J., Santiago Moreno, Julián, CSIC - Instituto Nacional de Investigación y Tecnología Agraria y Alimentaria (INIA), Galarza, Diego Andres [0000-0002-0266-5431], Bóveda, Paula [0000-0001-5749-4345], Toledano-Diaz, A. [0000-0001-6679-485X], Castaño, Cristina [0000-0003-1134-1436], Esteso, Milagros C. [0000-0002-8963-5736], López Sebastián, Antonio [0000-0001-8695-7441], Sánchez-Calabuig, M. J. [0000-0002-4280-992X], Santiago Moreno, Julián [0000-0001-5551-8120], Galarza, Diego Andres, Bóveda, Paula, Toledano-Díaz, A., Castaño, Cristina, Esteso, Milagros C., López Sebastián, Antonio, Sánchez-Calabuig, M. J., and Santiago Moreno, Julián

Abstract

This article describes the urinogenital condition of three female Iberian ibexes (Capra pyrenaica-one infertile 3-yr-old adult and two prepubertal animals aged 1 (PP1) and 2 (PP2) yr, respectively, all raised in captivity. All showed constant urinal dribbling, leading to ulcerative dermatitis in the vulvar area. Housed in a stable with other females, the adult did not become pregnant after male contact in either of two consecutive mating seasons. Vaginoscopy and laparoscopic exploration performed on the prepubertal females revealed abnormalities of the vagina and urinary bladder. Ultrasound examination revealed atrophy of the left kidney in the adult female and PP1, and of the right kidney in PP2, with degeneration of the renal pelvis. A paraovarian cyst with hydrosalpinx was also detected in the left oviduct of the adult female. Postmortem analysis of the adult and PP2, which shared a mother, confirmed an extramural single ectopic ureter with vaginal insertion associated with atrophy of the ipsilateral kidney. Though PP1 was officially unrelated to the latter animals, all three might have had a common ancestor in their lineages.

Published
2020

22. Use of native chicken breeds ( Gallus gallus domesticus ) for the development of suitable methods of Cantabrian capercaillie ( Tetrao urogallus cantabricus ) semen cryopreservation

Author

O'Brien, Emma, primary, Castaño, Cristina, additional, Toledano‐Díaz, Adolfo, additional, Caamaño, José Néstor, additional, Hidalgo, Carlos, additional, Fidalgo, Luis Eusebio, additional, López‐Beceiro, Ana María, additional, Esteso, Milagros Cristina, additional, Balsera, Ramón, additional, García‐Casado, Pedro, additional, Łukaszewicz, Ewa, additional, and Santiago‐Moreno, Julián, additional

Published
2022
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24. Seminal plasma amino acid profile in different breeds of chicken Role of seminal plasma on sperm cryoresistance

Author

Castaño, Cristina [0000-0003-1134-1436], Esteso, Milagros C. [0000-0002-8963-5736], García-Gil, María [0000-0003-2856-277X], Santiago Moreno, Julián [0000-0001-5551-8120], Toledano-Diaz, A. [0000-0001-6679-485X], Gutiérrez-Adán, Alfonso [0000-0001-9893-9179], López Sebastián, Antonio [0000-0001-8695-7441], Santiago Moreno, Julián, Bernal Juárez, Berenice, Pérez Cerezales, Serafín, Castaño, Cristina, Toledano-Díaz, A., Esteso, Milagros C., Gutiérrez-Adán, Alfonso, López Sebastián, Antonio, García-Gil, María, Woelders, Henri, Blesbois, E., Castaño, Cristina [0000-0003-1134-1436], Esteso, Milagros C. [0000-0002-8963-5736], García-Gil, María [0000-0003-2856-277X], Santiago Moreno, Julián [0000-0001-5551-8120], Toledano-Diaz, A. [0000-0001-6679-485X], Gutiérrez-Adán, Alfonso [0000-0001-9893-9179], López Sebastián, Antonio [0000-0001-8695-7441], Santiago Moreno, Julián, Bernal Juárez, Berenice, Pérez Cerezales, Serafín, Castaño, Cristina, Toledano-Díaz, A., Esteso, Milagros C., Gutiérrez-Adán, Alfonso, López Sebastián, Antonio, García-Gil, María, Woelders, Henri, and Blesbois, E.

Abstract

Seminal plasma is a key biological fluid that modulates sperm function in the reproduction process. However, its role in sperm biotechnologies is scarce in poultry. The aims of the present study were to study the amino acids profile and total proteins of seminal plasma in 12 Spanish chicken breeds and to investigate the role of seminal plasma on cryoresistance of rooster sperm. To investigate the role of seminal plasma on cryoresistance, diluted pooled semen samples were cryopreserved in the presence and absence of seminal plasma. Glutamic acid was the most abundant free amino acid in seminal plasma, followed by alanine, serine, valine, and glycine. There was an influence of breed (P<0.05) on the percentage of viable sperm after freezing-thawing of samples with seminal plasma. Cluster analysis revealed that White Prat, Black Castellana, Blue Andaluza, Quail Castellana, and Red-Barred Vasca returned the best freezing-thawing response (good freezers). There was a positive correlation between seminal plasma concentrations of valine, isoleucine lysine, leucine and post thaw viability. The evaluation of fertilization capacity of frozen-thawed semen from the breeds White Prat (‘good freezer’) and Black-Red Andaluza (‘bad freezer’) showed that good freezer had higher fertility (20/68, 29.4%) compared to bad freezer breed (14/76, 18.4%), even if the difference was not significant (P = 0.08). The TUNEL assay revealed that freezing/thawing procedures in presence of seminal plasma provoked higher DNA fragmentation in most of the breeds, with a positive correlation between seminal alanine, valine, isoleucine, methionine, leucine, tyrosine, phenylalanine concentrations and DNA integrity. DNA fragmentation was lower in absence of seminal plasma and the breed effect on sperm viability was highly reduced. It is concluded that specific seminal plasma amino acids were associated with post-thaw percentage of viable sperm and DNA integrity. The removal of seminal plasma decreases the v

Published
2019

25. Semen cryopreservation in black-footed (Spheniscus demersus) and gentoo (Pygoscelis papua) penguins Effects of thawing temperature on semen characteristics

Author

Castaño, Cristina [0000-0003-1134-1436], Martínez-Nevado, Eva [0000-0002-8994-4205], Esteso, Milagros C. [0000-0002-8963-5736], Santiago Moreno, Julián, Castaño, Cristina, Toledano-Díaz, A., Esteso, Milagros C., Martínez-Nevado, Eva, Gimeno-Martínez, J., López-Goya, A., Castaño, Cristina [0000-0003-1134-1436], Martínez-Nevado, Eva [0000-0002-8994-4205], Esteso, Milagros C. [0000-0002-8963-5736], Santiago Moreno, Julián, Castaño, Cristina, Toledano-Díaz, A., Esteso, Milagros C., Martínez-Nevado, Eva, Gimeno-Martínez, J., and López-Goya, A.

Abstract

In this study, there was an examination of the effect on the characteristics of cryopreserved black-footed (Spheniscus demersus) and gentoo (Pygoscelis papua) penguin semen, of thawing at 37 and 5 °C. For two consecutive years, semen was collected and frozen during the April-June period from six gentoo penguins, and during the October-November period from 13 black-footed penguins. After thawing, sperm motility variables were examined by computer-assisted sperm analysis. Propidium iodide and SYBR-14 were used as fluorochromes for the examination of membrane integrity. For the gentoo penguins, no differences were detected in the values of frozen-thawed semen characteristics after thawing at 37 or 5 °C. For the black-footed penguins, however, thawing at 5 °C resulted in greater values (P < 0.05) for straight-line velocity (VSL), average path velocity (VAP), linearity (LIN), straightness (STR), and wobble (WOB) as compared with thawing at 37 °C. After thawing at 37 ºC, there were greater values with gentoo penguin sperm for percentage motile sperm, progressive motility, curvilinear velocity (VCL), VSL VAP, LIN, STR, WOB and beat-cross frequency (BCF; P < 0.05) than that for black-footed penguin sperm. After thawing at 5 ºC, there were no differences in values for any variables between the two species. In conclusion, thawing temperature affects semen characteristics in a species-specific manner. The present data strongly suggest that cryopreservation procedures should be adapted for use with each penguin species. Cryopreserved black-footed penguin semen should be thawed after cryopreservation at 5 ºC, while that of gentoo penguins can be thawed at either 5 or 37 ºC.

Published
2019

28. Influence of circulating testosterone concentration on sperm cryoresistance: The ibex as an experimental model

Author

Bóveda, Paula, primary, Esteso, Milagros Cristina, additional, Velázquez, Rosario, additional, Castaño, Cristina, additional, Toledano‐Díaz, Adolfo, additional, López‐Sebastián, Antonio, additional, Mejía, Octavio, additional, Millán de la Blanca, María Gemma, additional, Ungerfeld, Rodolfo, additional, and Santiago‐Moreno, Julián, additional

Published
2021
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29. Slow and ultra-rapid freezing protocols for cryopreserving mouflon (Ovis musimon) and fallow deer (Dama dama) epididymal sperm

Author

Esteso, Milagros C. [0000-0002-8963-5736], Castaño, Cristina [0000-0003-1134-1436], Toledano-Diaz, A. [0000-0001-6679-485X], López Sebastián, Antonio [0000-0001-8695-7441], Ungerfeld, Rodolfo [0000-0003-4685-2105], Santiago Moreno, Julián [0000-0001-5551-8120], Bóveda, Paula, Esteso, Milagros C., Castaño, Cristina, Toledano-Díaz, A., López Sebastián, Antonio, Muñiz, A., Prieto, Paloma, Mejía, Octavio, Ungerfeld, Rodolfo, Santiago Moreno, Julián, Esteso, Milagros C. [0000-0002-8963-5736], Castaño, Cristina [0000-0003-1134-1436], Toledano-Diaz, A. [0000-0001-6679-485X], López Sebastián, Antonio [0000-0001-8695-7441], Ungerfeld, Rodolfo [0000-0003-4685-2105], Santiago Moreno, Julián [0000-0001-5551-8120], Bóveda, Paula, Esteso, Milagros C., Castaño, Cristina, Toledano-Díaz, A., López Sebastián, Antonio, Muñiz, A., Prieto, Paloma, Mejía, Octavio, Ungerfeld, Rodolfo, and Santiago Moreno, Julián

Abstract

This study examines the effectiveness of two methods for cryopreserving post-mortem epididymal sperm - conventional slow freezing employing a short equilibration time with glycerol, and ultra-rapid freezing - from the wild ruminant species Ovis musimon (mouflon) and Dama dama (fallow deer). A Tris-citric acid-glucose (TCG) + 12% egg yolk-based medium was used for the conventional slow freezing of the fallow deer sperm, whereas a Tes-Tris-glucose (TEST) + 6% egg yolk-based medium was used for the mouflon sperm. Glycerol was added to a final concentration of 5% to both media. The same diluents were used for ultra-rapid freezing but replacing the glycerol with 100 mM of sucrose. Sperm variables (motility, viability, acrosome integrity, membrane integrity, and morphological abnormalities) were analyzed before and after cryopreservation. Although values were generally better after the thawing of the conventionally cryopreserved sperm, total sperm motility (38.40 ± 4.44% in mouflon and 31.25 ± 3.37% in fallow deer) and total live sperm (47.19 ± 5.18% in mouflon and 43.13 ± 2.43% in fallow deer) were acceptable for the ultra-rapidly cooled sperm. Independent of the cryopreservation method, membrane integrity, acrosome integrity and the percentages of dead sperm and sperms with a damaged acrosome were better for the cryopreserved mouflon sperm than the fallow deer sperm (P < 0.05). Despite exerting a more harmful effect on sperm variables than conventional freezing, ultra-rapid freezing may be a useful alternative for the cryopreservation of these species' epididymal sperm in the field, as this simple technique does not require sophisticated equipment and expertise.

Published
2018

30. Fertilizing capacity of vitrified epididymal sperm from Iberian ibex (Capra pyrenaica)

Author

Castaño, Cristina [0000-0003-1134-1436], Rizos, Dimitrios [0000-0001-6813-3940], Esteso, Milagros C. [0000-0002-8963-5736], Pradiee, J., Sánchez-Calabuig, M. J., Castaño, Cristina, O'Brien, Emma, Esteso, Milagros C., Beltrán Breña, Paula, Maillo, V., Santiago Moreno, Julián, Rizos, Dimitrios, Castaño, Cristina [0000-0003-1134-1436], Rizos, Dimitrios [0000-0001-6813-3940], Esteso, Milagros C. [0000-0002-8963-5736], Pradiee, J., Sánchez-Calabuig, M. J., Castaño, Cristina, O'Brien, Emma, Esteso, Milagros C., Beltrán Breña, Paula, Maillo, V., Santiago Moreno, Julián, and Rizos, Dimitrios

Abstract

In this study, we successfully described for the first time a vitrification of epididymal Iberian ibex spermatozoa. Spermatozoa from epididymis were obtained from 15 Iberian ibex. The right epididymis' semen sample was vitrified and the left one was frozen. After thawing/warming, samples were selected by density gradient. Sperm characteristics from each treatment were evaluated. To test the spermatozoa fertilization ability, heterologous IVF was carried out using bovine oocytes. Despite of the observation of a decrease of about 40% for motility sperm between pre-freezing and post-thawing (75.0 ± 5.2 and 45.0 ± 6.0) and pre-vitrification and post-warming (78.2 ± 5.2 and 33.9 ± 6.2) (P < .05), after the washing, an improvement of sperm motility was found when using the vitrification treatment compared to frozen-thawed. Heterologous IVF showed that Iberian Ibex spermatozoa, either frozen-thawed or vitrified-warmed, were equally capable of penetrating ZP intact bovine oocytes, leading to pronuclear formation (%) and hybrid embryo cleavage (%), (31.3 ± 27.2 and 45.1 ± 24.4, respectively). As expected, in the homologous IVF group, higher percentages of penetration, pronuclei formation and cleavage were found compared to heterologous groups using Iberian ibex frozen and vitrified sperm (P < 0,5). The highest pronuclei formation was found after 20 h post insemination in both heterologous IVF groups (30.2 ± 6.7 and 31.7 ± 21.5 thawed and vitrified group). Consequently, the cleavage rate (48 h) followed the same results to homologous and thawed and vitrified groups (76.1 ± 15.9; 31.3 ± 27.2 and 45.1 ± 24.4, respectively) (P < .05). In conclusion, Iberian ibex sperm vitrification is a promising and useful alternative to conventional methods resulting in good quality spermatozoa post-thaw, and an adequate in vitro fertilizing ability.

Published
2018

31. Effect of two cooling protocols on the post-thaw characteristics of Iberian ibex sperms

Author

Castaño, Cristina [0000-0003-1134-1436], Esteso, Milagros C. [0000-0002-8963-5736], López Sebastián, Antonio [0000-0001-8695-7441], Santiago Moreno, Julián [0000-0001-5551-8120], Esteso, Milagros C., Toledano-Díaz, A., Castaño, Cristina, Pradiee, J., López Sebastián, Antonio, Santiago Moreno, Julián, Castaño, Cristina [0000-0003-1134-1436], Esteso, Milagros C. [0000-0002-8963-5736], López Sebastián, Antonio [0000-0001-8695-7441], Santiago Moreno, Julián [0000-0001-5551-8120], Esteso, Milagros C., Toledano-Díaz, A., Castaño, Cristina, Pradiee, J., López Sebastián, Antonio, and Santiago Moreno, Julián

Abstract

The rate at which lethal intracellular ice forms during sperm cryopreservation is highly dependent on the cooling protocol. The present work compares two cooling protocols for use with Iberian ibex (Capra pyrenaica) sperm by assessing the effects on the motility, viability, and size of frozen-thawed sperm cells. Ejaculates, obtained from six adult ibex males via transrectal, ultrasound-guided massage of the accessory sex glands plus electroejaculation if necessary, were cooled via either 1) Protocol 1 (decelerating cooling), involving cooling in liquid nitrogen vapor from 5 °C to -35 °C (40 °C/min), from -35 °C to -65 °C (17 °C/min), and then from -65 °C to -85 °C (3 °C/min); or 2) Protocol 2 (accelerating cooling) involving cooling in a biological freezer from 5 °C to -5 °C (4 °C/min), from -5 °C to -110 °C (25 °C/min), and then from -110 °C to -140 °C (35 °C/min). Compared to fresh ejaculates, sperm quality at thawing was found to be reduced by both protocols (p < .05), but especially by Protocol 1. Sperm head size was also significantly reduced by both protocols, although the Protocol 1 sperm heads were also significantly smaller than those of Protocol 2 sperms heads (p < .05). In fresh sperm samples, clustering analyses revealed two subpopulations of sperms with different morphometric characteristics, SP1 with larger cells, and SP2 with smaller cells. Both cooling protocols caused reduction in the proportion of SP1 cells, and an increase in the proportion of SP2 cells. In conclusion, the decelerating cooling protocol (Protocol 1) caused greater cryodamage to the sperm cells than the accelerating protocol (Protocol 2).

Published
2018

32. The percentage of egg yolk in the freezing media affects mouflon (Ovis musimon) epididymal sperm cryosurvival

Author

Martínez-Fresneda, Lucía [0000-0002-0967-8593], Esteso, Milagros C. [0000-0002-8963-5736], Toledano-Diaz, A. [0000-0001-6679-485X], Castaño, Cristina [0000-0003-1134-1436], López Sebastián, Antonio [0000-0001-8695-7441], García-Vázquez, Francisco Alberto [0000-0001-7665-3858], Santiago Moreno, Julián [0000-0001-5551-8120], Velázquez, Rosario [0009-0009-2115-4715], Martínez-Fresneda, Lucía, Esteso, Milagros C., Toledano-Díaz, A., Castaño, Cristina, Velázquez, Rosario, López Sebastián, Antonio, Prieto, Paloma, García-Vázquez, Francisco Alberto, Santiago Moreno, Julián, Martínez-Fresneda, Lucía [0000-0002-0967-8593], Esteso, Milagros C. [0000-0002-8963-5736], Toledano-Diaz, A. [0000-0001-6679-485X], Castaño, Cristina [0000-0003-1134-1436], López Sebastián, Antonio [0000-0001-8695-7441], García-Vázquez, Francisco Alberto [0000-0001-7665-3858], Santiago Moreno, Julián [0000-0001-5551-8120], Velázquez, Rosario [0009-0009-2115-4715], Martínez-Fresneda, Lucía, Esteso, Milagros C., Toledano-Díaz, A., Castaño, Cristina, Velázquez, Rosario, López Sebastián, Antonio, Prieto, Paloma, García-Vázquez, Francisco Alberto, and Santiago Moreno, Julián

Abstract

Sperm cryopreservation protocols are not well defined in many wild species such as the mouflon. The aim was to study the effect of different concentrations of EY on mouflon epididymal sperm cryosurvival. Samples were collected by the flushing method and cryopreserved by the conventional freezing technique in straws using a TEST (TES, Tris, glucose) 5% v/v glycerol medium containing either 6% v/v (n=16) or 12% v/v (n=13) clarified EY. The membrane integrity, acrosome integrity, motility, and morphological abnormalities were assessed in fresh and frozen/thawed samples. Fresh sperm quality parameters did not differ between groups except for the acrosome integrity that was lower in the TEST-6% EY than in the TEST-12% EY group (88.9 ± 2.1% vs 94.7 ± 0.8%). Membrane integrity (31.6 ± 4.6% vs 11.6 ± 4.5%), total motility (32.8 ± 4.6% vs 17.2 ± 5.6%), progressive motility (13.3 ± 2.7% vs 6.1 ± 2.9) were higher in frozen-thawed sperm with TEST-6% EY than with TEST-12% EY (p<0.05). Other motility parameters such as curvilinear velocity, straight-line velocity, average path velocity and amplitude of lateral head displacement were also higher (p<0.05) in frozen-thawed sperm with TEST-6% EY. Frozen-thawed acrosome integrity (85.1 ± 3.3% vs 91.9 ± 2.3) and morphological abnormalities (34.0 ± 3.7% vs 29.1 ± 3.6%) did not differ between extenders. In conclusion, high EY concentration had detrimental effects on post-thaw quality parameters, therefore the use of TEST based extender containing 6% EY is recommended for the cryopreservation of mouflon epididymal sperm.

Published
2018

34. Unilateral single vaginal ectopic ureter with ipsilateral hypoplastic and degenerated kidney associated with infertility in iberian ibex (capra pyrenaica) does

Author

Galarza Lucero, Diego Andres, Bóveda Gómez, Paula, Toledano Díez, Adolfo, Castaño, Cristina, Esteso, Milagros, López Sebastián, Antonio, Sánchez Calabuig, María Jesús, Santiago Moreno, Julián, Galarza Lucero, Diego Andres, Bóveda Gómez, Paula, Toledano Díez, Adolfo, Castaño, Cristina, Esteso, Milagros, López Sebastián, Antonio, Sánchez Calabuig, María Jesús, and Santiago Moreno, Julián

Abstract

This article describes the urinogenital condition of three female Iberian ibexes (Capra pyrenaica—one infertile 3-yr-old adult and two prepubertal animals aged 1 (PP1) and 2 (PP2) yr, respectively, all raised in captivity. All showed constant urinal dribbling, leading to ulcerative dermatitis in the vulvar area. Housed in a stable with other females, the adult did not become pregnant after male contact in either of two consecutive mating seasons. Vaginoscopy and laparoscopic exploration performed on the prepubertal females revealed abnormalities of the vagina and urinary bladder. Ultrasound examination revealed atrophy of the left kidney in the adult female and PP1, and of the right kidney in PP2, with degeneration of the renal pelvis. A paraovarian cyst with hydrosalpinx was also detected in the left oviduct of the adult female. Postmortem analysis of the adult and PP2, which shared amother, confirmed an extramural single ectopic ureter with vaginal insertion associated with atrophy of the ipsilateral kidney. Though PP1 was officially unrelated to the latter animals, all three might have had a common ancestor in their lineages.

Published
2020

35. Optimization of sperm cryopreservation protocol for peregrine falcon (Falco peregrinus)

Author

Ministerio de Economía y Competitividad (España), European Commission, Cardoso, Beatriz, Sánchez-Ajofrín, Irene, Castaño, Cristina, García-Álvarez, Olga, Esteso, Milagros C., Maroto-Morales, Alejandro, Iniesta-Cuerda, María, Garde, José Julián, Santiago-Moreno, Julián, Soler, Ana J., Ministerio de Economía y Competitividad (España), European Commission, Cardoso, Beatriz, Sánchez-Ajofrín, Irene, Castaño, Cristina, García-Álvarez, Olga, Esteso, Milagros C., Maroto-Morales, Alejandro, Iniesta-Cuerda, María, Garde, José Julián, Santiago-Moreno, Julián, and Soler, Ana J.

Abstract

Sperm cryopreservation is a complex process that needs to be adapted to wild and domestic avian species to ensure proper efficiency. Because of its accessibility, the peregrine falcon may be used as a good model for studying other raptor species. To find the most optimal cryopreservation protocol for peregrine falcon ejaculates, sperm parameters such as motility, viability, DNA fragmentation, acrosome integrity, and mitochondrial activity were analyzed under different conditions by varying the freezing method (slow freezing in straws vs. ultrarapid freezing in pellets), thawing conditions (37 °C for 30 s vs. 5 °C for 1 min), type of cryoprotectant (DMA vs. DMSO), and concentration of DMSO (4% vs. 8%). Results show that slow cryopreservation in straws yielded greater percentages (p < 0.05) of motile spermatozoa (22.5% ± 4.4% vs. 0.0% ± 4.1%), viable spermatozoa with intact acrosomes (84.6% ± 4.3% vs. 77.4% ± 4.3%), and spermatozoa with active mitochondria (41.0% ± 6.7% vs.12.8% ± 6.7%), compared with those obtained by the ultrarapid freezing in pellets. However, no differences were found between different thawing conditions. Moreover, all sperm motility parameters were greater (p < 0.05) when DMSO was used during freezing compared with DMA, although the use of 3% and 8% DMSO produced similar results. In conclusion, these results represent important progress in the study of falcon semen cryopreservation protocol, highlighting the crucial steps of the process and the most suitable conditions.

Published
2020

36. Sperm Cryopreservation in American Flamingo (Phoenicopterus Ruber): Influence of Cryoprotectants and Seminal Plasma Removal

Author

Millán de la Blanca, María Gemma, primary, Martínez-Nevado, Eva, additional, Castaño, Cristina, additional, García, Juncal, additional, Bernal, Berenice, additional, Toledano-Díaz, Adolfo, additional, Esteso, Milagros Cristina, additional, Bóveda, Paula, additional, Martínez-Fresneda, Lucía, additional, López-Sebastián, Antonio, additional, and Santiago-Moreno, Julián, additional

Published
2021
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38. Cryopreservation of ferret ( Mustela putorius furo ) sperm collected by rectal massage and electroejaculation: Comparison of a decelerating and an accelerating freezing rate protocol

Author

Toledano‐Díaz, Adolfo, primary, Castaño, Cristina, additional, Velázquez, Rosario, additional, Bóveda, Paula, additional, López‐Sebastián, Antonio, additional, Martínez‐Nevado, Eva, additional, Villaverde‐Morcillo, Silvia, additional, Esteso, Milagros C., additional, and Santiago‐Moreno, Julián, additional

Published
2020
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40. UNILATERAL SINGLE VAGINAL ECTOPIC URETER WITH IPSILATERAL HYPOPLASTIC AND DEGENERATED KIDNEY ASSOCIATED WITH INFERTILITY IN IBERIAN IBEX (CAPRA PYRENAICA) DOES

Author

Lucero, Diego Galarza, primary, Gómez, Paula Bóveda, additional, Toledano-Díaz, Adolfo, additional, Castaño, Cristina, additional, Esteso, Milagros, additional, López-Sebastián, Antonio, additional, Sánchez-Calabuig, María Jesús, additional, and Santiago-Moreno, Julián, additional

Published
2020
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42. Conventional slow freezing cryopreserves mouflon spermatozoa better than vitrification

Author

Castaño, Cristina [0000-0003-1134-1436], Esteso, Milagros C. [0000-0002-8963-5736], López Sebastián, Antonio [0000-0001-8695-7441], Pradiee, J., Esteso, Milagros C., Castaño, Cristina, Toledano-Díaz, A., López Sebastián, Antonio, Guerra, Rafael, Santiago Moreno, Julián, Castaño, Cristina [0000-0003-1134-1436], Esteso, Milagros C. [0000-0002-8963-5736], López Sebastián, Antonio [0000-0001-8695-7441], Pradiee, J., Esteso, Milagros C., Castaño, Cristina, Toledano-Díaz, A., López Sebastián, Antonio, Guerra, Rafael, and Santiago Moreno, Julián

Abstract

This work examines the effectiveness of a TCG (Tris, citric acid, glucose, 6% egg yolk and 5% glycerol) and a TEST (TES, Tris, glucose, 6% egg yolk and 5% glycerol) sperm extender in the freezing of mouflon spermatozoa at slow cooling rates, using different pre-freezing equilibration times (2–3 hr). It also examines the tolerance of mouflon spermatozoa to different concentrations of cryoprotectants (5, 10, 20% glycerol; 5%, 10%, 20% dimethyl sulfoxide; 6% polyvinylpyrrolidone) and/or sucrose (100, 300, 500 mm). The highest quality (p <.01) thawed spermatozoa were obtained when using the TEST extender and an equilibration time of 3 hr. Sperm motility and membrane integrity were strongly reduced when using rapid freezing rates (60–85°C min−1), independent of the concentration of cryoprotectants. The lowest sucrose concentration (100 mm) provided the highest (p <.05) percentage of motile spermatozoa and live spermatozoa with an intact acrosome. Vitrified–warmed sperm variables were at their best when the spermatozoa was diluted in TCG–6% egg yolk + 100 mm sucrose and warmed at 60°C. Slow warming at 37°C strongly reduced (p <.05) sperm motility and viability. However, sperm vitrification returned lower fertility, sperm motility and sperm viability values than conventional sperm freezing. © 2016 Blackwell Verlag GmbH

Published
2017

43. Seminal plasma removal by density-gradient centrifugation is superior for goat sperm preservation compared with classical sperm washing

Author

Santiago Moreno, Julián [0000-0001-5551-8120], Esteso, Milagros C. [0000-0002-8963-5736], Castaño, Cristina [0000-0003-1134-1436], Toledano-Diaz, A. [0000-0001-6679-485X], López Sebastián, Antonio [0000-0001-8695-7441], Santiago Moreno, Julián, Esteso, Milagros C., Castaño, Cristina, Toledano-Díaz, A., Delgadillo, J. A., López Sebastián, Antonio, Santiago Moreno, Julián [0000-0001-5551-8120], Esteso, Milagros C. [0000-0002-8963-5736], Castaño, Cristina [0000-0003-1134-1436], Toledano-Diaz, A. [0000-0001-6679-485X], López Sebastián, Antonio [0000-0001-8695-7441], Santiago Moreno, Julián, Esteso, Milagros C., Castaño, Cristina, Toledano-Díaz, A., Delgadillo, J. A., and López Sebastián, Antonio

Abstract

Seminal plasma removal is routine in goat sperm cryopreservation protocols. The classical washing procedure designed to accomplish this usually leaves the pellet resulting from use of this procedure contaminated with dead sperm, debris, and cells other than sperm. This contamination negatively affects viability of sperm after cryopreservation. The present research was conducted to compare the effect on chilled and frozen-thawed goat sperm of the classical washing method to that of a selective washing method involving density gradient centrifugation (DGC). In the first experiment, sperm variables were measured in freshly collected sperm, and again after its washing with both methods and chilling at 5 °C for 0, 3, 24, 48, 72 or 96 h. The DGC-washed sperm had greater (P < 0.01) straight line velocity (VSL), average path velocity (VAP) and progression ratio values at all chilling times. The amplitude of lateral head displacement (ALH) was, however, less (P < 0.001) in the DGC-washed sperm at all chilling times. There was a negative correlation (P < 0.05) between ALH and VSL. In the second experiment involving the freezing-thawing of sperm washed by using either method, aliquots were post-wash diluted with a Tris-citric acid/glucose/egg yolk/glycerol-based medium and frozen in liquid nitrogen for 5 days. After thawing, neither the VCL, VSL nor VAP of the DGC-washed samples were affected, whereas the traditionally washed samples had less motility. In conclusion, the use of DGC was associated with enhanced sperm motility variables after chilling and freezing-thawing. This procedure would, therefore, be a useful means of removing seminal plasma from goat semen and obtaining greater quality sperm for insemination purposes. © 2017

Published
2017

44. Successful chilling of red-legged partridge (Alectoris rufa) sperm for use in artificial insemination

Author

Santiago Moreno, Julián [0000-0001-5551-8120], Castaño, Cristina [0000-0003-1134-1436], Toledano-Diaz, A. [0000-0001-6679-485X], Esteso, Milagros C. [0000-0002-8963-5736], López Sebastián, Antonio [0000-0001-8695-7441], García Dávila, Sara [0000-0003-4152-8373], García-Gil, María [0000-0003-2856-277X], Santiago Moreno, Julián, Castaño, Cristina, Toledano-Díaz, A., Esteso, Milagros C., López Sebastián, Antonio, Villaverde-Morcillo, S., García Dávila, Sara, García-Gil, María, Blesbois, E., Santiago Moreno, Julián [0000-0001-5551-8120], Castaño, Cristina [0000-0003-1134-1436], Toledano-Diaz, A. [0000-0001-6679-485X], Esteso, Milagros C. [0000-0002-8963-5736], López Sebastián, Antonio [0000-0001-8695-7441], García Dávila, Sara [0000-0003-4152-8373], García-Gil, María [0000-0003-2856-277X], Santiago Moreno, Julián, Castaño, Cristina, Toledano-Díaz, A., Esteso, Milagros C., López Sebastián, Antonio, Villaverde-Morcillo, S., García Dávila, Sara, García-Gil, María, and Blesbois, E.

Abstract

The fertilizing capacity of pure, fresh avian semen may disappear in just half an hour, hindering its successful use in artificial insemination (AI) projects. Longer storage requires the use of infra-physiological temperatures and of semen diluents that help preserve the spermatozoa but that do not interfere with their fertilizing capacity. This study examines the effect on sperm quality of storing red-legged partridge sperm for 3 h at 5°C with 2 different semen extenders: 1) a medium referred to as L&R-84, composed of sodium glutamate, glucose, magnesium acetate, potassium acetate, and polyvinylpyrrolidone, and 2) Lake 7.1 medium, composed of sodium glutamate, glucose, magnesium acetate, potassium citrate, and N,N-Bis(2-hydroxyethyl)taurine (BES). Extending with L&R-84 returned better curvilinear velocity (P < 0.01), straight-line velocity (P < 0.01), average path velocity (P < 0.01), linearity (P < 0.05), straightness (P < 0.05), and wobble (P < 0.05) values, while extending with the Lake 7.1 medium was associated with higher percentages (P < 0.001) of motile sperm. The fertility rate was higher (P < 0.05) when birds were inseminated with L&R-84-extended sperm than with Lake 7.1-extended sperm. The mean number of penetrations of perivitelline layer samples (taken from above the germinal disc) was also higher for the L&R-84-extended sperm (P < 0.05). These results show L&R-84 can be recommended as an extender for red-legged partridge semen to be stored for at least 3 h at 5°C.

Published
2017

45. Aplicación de las técnicas de reproducción asistida a la conservación de la variedad negra de la raza Manchega

Author

Benítez, Martín J., Mora, Antonio I., Pérez Sempere-M., José-I., Esteso, Milagros, Fernández, Rocio, Martínez Pastor, Felipe, Montoro, Vidal, Garde López-Brea, Julián, Pérez Guzmán, María Dolores, Soler, Ana J., Arias, Ramón, Biologia Celular, and Facultad de Ciencias Biologicas y Ambientales

Subjects
Biotecnología, Reproducción asistida, Ganado ovino, Veterinaria, Manchega (Raza ovina)
Abstract

P. 102-104 Aplicación de las técnicas de reproducción asistida a la conservación de la variedad negra de la raza Manchega SI

Published
2019

46. Refrigerated Storage of Red Deer Epididymal Spermatozoa in the Epididymis, Diluted and with Vitamin C Supplementation

Author

Fernández Santos, María Rocío, Biologia Celular, Fernández Santos, María Rocío, Domínguez Rebolledo, Álvaro Efrén, Esteso, Milagros, Garde López-Brea, Julián, Martínez Pastor, Felipe, Fernández Santos, María Rocío, Biologia Celular, Fernández Santos, María Rocío, Domínguez Rebolledo, Álvaro Efrén, Esteso, Milagros, Garde López-Brea, Julián, and Martínez Pastor, Felipe

Abstract

We have approached the problem of refrigerated storage of epididymal sperm samples from red deer by comparing three options: storing the genital (testicles within the scrotum), diluting the semen in extender or diluting the semen in extender supplemented with an anti‐oxidant. Twenty‐nine pairs of testes were collected. Spermatozoa from one of each of the pairs were immediately recovered, and diluted to 400 × 106 sperm/ml in Tris‐citrate‐fructose with 20% egg yolk. Control group was stored as such, and Anti‐oxidant group was supplemented with 0.8 mm vitamin C. The remaining epididymides and the diluted samples were stored at 5°C and spermatozoa were analysed at 0, 24, 96 and 192 h for: motility [computer‐assisted semen analysis (CASA)], acrosomal integrity, sperm viability (eosine/nigrosine staining), normal tails and chromatin status [sperm chromatin structure assay (SCSA)]. In general, seminal quality decreased with storage time. Vitamin C supported progressive motility better at 24 h (median 42% vs 23% Control and 15% epididymis), reduced the incidence of tail abnormalities and protected chromatin. Storing the semen in the epididymis slowed down motility loss, but slightly increased the occurrence of tail abnormalities and viability was lower at 192 h. However, regarding chromatin status, sperm stored in the epididymis was protected similarly to those diluted in the medium supplemented with vitamin C. Although the differences between the three groups were small, there were some advantages in supplementing the extender with vitamin C. Besides, refrigerating the epididymis may be a good option when immediate processing is not available.

Published
2019

47. Sperm characteristics and in vitro fertilization ability of thawed spermatozoa from Black Manchega ram: Electroejaculation and postmortem collection

Author

García Álvarez, Olga, Biologia Celular, García Álvarez, Olga, Maroto Morales, Alejandro, Martínez Pastor, Felipe, Garde López-Brea, Julián, Ramón Fernández, Manuel, Fernández Santos, María Rocío, Esteso, Milagros, Pérez Guzmán, María Dolores, Soler, Ana J., García Álvarez, Olga, Biologia Celular, García Álvarez, Olga, Maroto Morales, Alejandro, Martínez Pastor, Felipe, Garde López-Brea, Julián, Ramón Fernández, Manuel, Fernández Santos, María Rocío, Esteso, Milagros, Pérez Guzmán, María Dolores, and Soler, Ana J.

Abstract

The aim of this study was to assess two models of sperm collection on the quality and fertility of thawed spermatozoa from Black Manchega rams, a threatened breed. Sperm samples were collected by electroejaculation and postmortem from each male. Samples were diluted with Biladyl and frozen. Motility (subjective and objective by means of computer-assisted semen analysis), membrane integrity, and acrosomal status (microscopy) were assessed on fresh and thawed semen; plasmalemma integrity, mitochondrial membrane potential, DNA integrity, and acrosomal status were evaluated by flow cytometry on thawed semen. Thawed spermatozoa were used in a heterologous in vitro fertilization test. After thawing, the proportion of live spermatozoa with intact membrane (YO-PRO-1−/PI−) was higher for postmortem samples (P < 0.001), although the ratio of YO-PRO-1− spermatozoa within the PI− population was higher for ejaculated samples (P = 0.007). Likewise, the proportion of live spermatozoa having high mitochondrial membrane potential (MitoTracker+) and intact acrosomes (PNA−) was higher for postmortem samples (P < 0.001 and P < 0.001, respectively). Considering only live spermatozoa, the ratio of MitoTracker+/PNA− cells was higher for electroejaculated samples (P = 0.026 and P = 0.003). Both electroejaculated and postmortem samples fertilized oocytes. Nevertheless, electroejaculated samples yielded a higher percentage of hybrid embryos (P = 0.041). In conclusion, although postmortem spermatozoa had better sperm quality after thawing, electroejaculated spermatozoa showed higher ratios for sperm quality when only the live population was considered. Electroejaculated and postmortem samples might be used for germplasm banking of this threatened breed, but the fertility of postmortem spermatozoa might be lower.

Published
2019

48. Sperm parameters on Iberian red deer: Electroejaculation and post-mortem collection

Author

Martínez, A. F., Biologia Celular, Martínez, A. F., Martínez Pastor, Felipe, Álvarez García, Mercedes, Fernández Santos, María Rocío, Esteso, Milagros, Paz Cabello, Paulino de, Garde López-Brea, Julián, Anel Rodríguez, Luis, Martínez, A. F., Biologia Celular, Martínez, A. F., Martínez Pastor, Felipe, Álvarez García, Mercedes, Fernández Santos, María Rocío, Esteso, Milagros, Paz Cabello, Paulino de, Garde López-Brea, Julián, and Anel Rodríguez, Luis

Abstract

Artificial reproductive technologies (ART) for cervids have improved, but a need remains for the collection of basic data. We studied two models of sperm collection in Iberian red deer, post-mortem (PM) in a wild population (179 samples) and by electroejaculation (EE) in a farmed population (37 samples), recording: testicular and epididymal weight, testicular diameter, sperm quantity, pH and osmolality and spermatozoa quality (motility by CASA, abnormal forms, cytoplasmic droplets, viability and acrosomal status). We tested the relationship of these parameters with stag age and compared the two models (PM and EE; medians showed). Genitalia parameters were linearly related to stag age (testicular diameter: 31.5–50.5 mm for 2–9 years). Total number of spermatozoa collected were PM: 2.5 × 109 and EE: 3.6 × 109 (P > 0.05), increasing with age only for PM. We found a positive relationship between testicular size and spermatozoa collected for PM. Osmolality and pH were PM: 6.28 and 378 mOsm/kg; EE: 7.63 and 309 mOsm/kg (P < 0.05). The pH increased with age only for EE. Percentage of motile spermatozoa was similar for PM and EE, but motility quality was lower for PM. Abnormal forms, proximal and distal droplets were lower for EE (22%, 1.3%, 1.5% vs. PM: 23%, 4.3%, 83%). Viability was similar (74%) and intact acrosomes were higher for EE (97% vs. 89%). Both PM and EE samples could be used for germplasm banking. This study contributes with new data on red deer spermatology and for the development of ART in cervids.

Published
2019

49. Seminal plasma amino acid profile in different breeds of chicken : Role of seminal plasma on sperm cryoresistance

Author

Santiago-Moreno, Julián, Bernal, Berenice, Pérez-Cerezales, Serafín, Castaño, Cristina, Toledano-Díaz, Adolfo, Esteso, Milagros C., Gutiérrez-Adán, Alfonso, López-Sebastián, Antonio, Gil, María G., Woelders, Henri, Blesbois, Elisabeth, Santiago-Moreno, Julián, Bernal, Berenice, Pérez-Cerezales, Serafín, Castaño, Cristina, Toledano-Díaz, Adolfo, Esteso, Milagros C., Gutiérrez-Adán, Alfonso, López-Sebastián, Antonio, Gil, María G., Woelders, Henri, and Blesbois, Elisabeth

Abstract

Seminal plasma is a key biological fluid that modulates sperm function in the reproduction process. However, its role in sperm biotechnologies is scarce in poultry. The aims of the present study were to study the amino acids profile and total proteins of seminal plasma in 12 Spanish chicken breeds and to investigate the role of seminal plasma on cryoresistance of rooster sperm. To investigate the role of seminal plasma on cryoresistance, diluted pooled semen samples were cryopreserved in the presence and absence of seminal plasma. Glutamic acid was the most abundant free amino acid in seminal plasma, followed by alanine, serine, valine, and glycine. There was an influence of breed (P<0.05) on the percentage of viable sperm after freezing-thawing of samples with seminal plasma. Cluster analysis revealed that White Prat, Black Castellana, Blue Andaluza, Quail Castellana, and Red-Barred Vasca returned the best freezing-thawing response (good freezers). There was a positive correlation between seminal plasma concentrations of valine, isoleucine lysine, leucine and post thaw viability. The evaluation of fertilization capacity of frozen-thawed semen from the breeds White Prat (‘good freezer’) and Black-Red Andaluza (‘bad freezer’) showed that good freezer had higher fertility (20/68, 29.4%) compared to bad freezer breed (14/76, 18.4%), even if the difference was not significant (P = 0.08). The TUNEL assay revealed that freezing/thawing procedures in presence of seminal plasma provoked higher DNA fragmentation in most of the breeds, with a positive correlation between seminal alanine, valine, isoleucine, methionine, leucine, tyrosine, phenylalanine concentrations and DNA integrity. DNA fragmentation was lower in absence of seminal plasma and the breed effect on sperm viability was highly reduced. It is concluded that specific seminal plasma amino acids were associated with post-thaw percentage of viable sperm and DNA integrity. The removal of seminal plasma decreases th

Published
2019

50. Refrigerated Storage of Red Deer Epididymal Spermatozoa in the Epididymis, Diluted and with Vitamin C Supplementation

Author

Biologia Celular, Fernández Santos, María Rocío, Domínguez Rebolledo, Álvaro Efrén, Esteso, Milagros, Garde López-Brea, Julián, Martínez Pastor, Felipe, Biologia Celular, Fernández Santos, María Rocío, Domínguez Rebolledo, Álvaro Efrén, Esteso, Milagros, Garde López-Brea, Julián, and Martínez Pastor, Felipe

Abstract

We have approached the problem of refrigerated storage of epididymal sperm samples from red deer by comparing three options: storing the genital (testicles within the scrotum), diluting the semen in extender or diluting the semen in extender supplemented with an anti‐oxidant. Twenty‐nine pairs of testes were collected. Spermatozoa from one of each of the pairs were immediately recovered, and diluted to 400 × 106 sperm/ml in Tris‐citrate‐fructose with 20% egg yolk. Control group was stored as such, and Anti‐oxidant group was supplemented with 0.8 mm vitamin C. The remaining epididymides and the diluted samples were stored at 5°C and spermatozoa were analysed at 0, 24, 96 and 192 h for: motility [computer‐assisted semen analysis (CASA)], acrosomal integrity, sperm viability (eosine/nigrosine staining), normal tails and chromatin status [sperm chromatin structure assay (SCSA)]. In general, seminal quality decreased with storage time. Vitamin C supported progressive motility better at 24 h (median 42% vs 23% Control and 15% epididymis), reduced the incidence of tail abnormalities and protected chromatin. Storing the semen in the epididymis slowed down motility loss, but slightly increased the occurrence of tail abnormalities and viability was lower at 192 h. However, regarding chromatin status, sperm stored in the epididymis was protected similarly to those diluted in the medium supplemented with vitamin C. Although the differences between the three groups were small, there were some advantages in supplementing the extender with vitamin C. Besides, refrigerating the epididymis may be a good option when immediate processing is not available.

Published
2019

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