RESUMO
O tecido testicular contém células germinativas, que possuem potencial para se desenvolver em espermatozoides viáveis por meio do cultivo in vitro ou xenotransplante, sendo uma alternativa interessante a ser utilizada na formação de biobancos. Esta revisão compila as atualizações, desafios e perspectivas relacionadas às técnicas de criopreservação e cultivo de tecido testicular como estratégia para a conservação de espécies mamíferas. O tecido testicular pode ser obtido tanto de indivíduos adultos como pré púberes, seja após orquiectomia ou até mesmo após a sua morte. O tecido fragmentado pode ser criopreservado por congelação lenta ou rápida e por métodos de vitrificação. Os crioprotetores são indispensáveis durante a criopreservação e podem variar o tipo e concentração de acordo com a espécie. Com os avanços da criopreservação deste material, espermatozoides podem ser obtidos por transplante de fragmentos testiculares ou células germinativas isoladas em camundongos imunodeficientes. No entanto, a obtenção de espermatozoides no cultivo in vitro ainda é um desafio.(AU)
The testicular tissue contains germ cells, which have the potential to develop into viable spermatozoa through in vitro culture or xenotransplantation, being an interesting alternative to be used in the formation of biobanks. This review compiles updates, challenges and perspectives related to cryopreservation techniques and testicular tissue culture as a strategy for the conservation of mammalian species. Testicular tissue can be obtained from both adult and pre-pubertal individuals, either after orchiectomy or even after their death. Fragmented tissue can be cryopreserved by slow or fast freezing and by vitrification methods. Cryoprotectants are indispensable during cryopreservation and may vary in type and concentration according to the species. With advances in cryopreservation of this material, spermatozoa can be obtained by transplanting testicular fragments or isolated germ cells into immunodeficient mice. However, obtaining spermatozoa in in vitro culture is still a challenge.(AU)
Assuntos
Animais , Masculino , Criopreservação/veterinária , Mamíferos/fisiologia , Espermatogênese , Crioprotetores , Células GerminativasRESUMO
Resumen La crioconservación es una herramienta biotecnológica que en peces está orientada principalmente a la conservación criogénica de semen como estrategia de preservación del recurso genético y a su uso para la producción de alevinos con fines diferentes. Actualmente, los protocolos de crioconservación seminal en peces de agua dulce establecen una amplia variedad de procedimientos cuya efectividad se basa en aspectos ligados a la calidad seminal post-descongelación y la fertilidad, así como su relación con el desarrollo de la progenie. El efecto de la conservación del semen en nitrógeno líquido por periodos amplios de tiempo también toma importancia en ésta biotecnología. Por lo anterior, el objetivo de la presente revisión es describir aspectos biotecnológicos, celulares y bioquímicos asociados al proceso de crioconservación seminal en peces dulceacuícolas, resaltando los avances, las limitaciones y sus perspectivas.
Abstract Cryopreservation is a biotechnological tool that in fish is mainly aimed at cryogenic conservation of semen as a strategy for preserving the genetic resource and its use for the production of fingerlings with different purposes. Currently, seminal cryopreservation protocols in freshwater fish establish a wide variety of procedures whose effectiveness is based on aspects linked to seminal post-thaw quality and fertility, as well as its relationship with the development of the progeny. The effect of preserving semen in liquid nitrogen for extended periods of time also plays an important role in this biotechnology. Therefore, the objective of this review is to describe biotechnological, cellular and biochemical aspects associated with the seminal cryopreservation process in freshwater fish, highlighting the advances, limitations and perspectives.
Resumo A criopreservação é uma ferramenta biotecnológica que em peixes visa principalmente a conservação criogênica do sêmen como estratégia para a preservação do recurso genético e sua utilização para a produção de alevinos para diferentes fins. Atualmente, os protocolos de criopreservação seminal em peixes de água doce estabelecem uma ampla variedade de procedimentos cuja eficácia se baseia em aspectos relacionados à qualidade e fertilidade pós-descongelamento seminal, bem como sua relação com o desenvolvimento da progênie. O efeito da preservação do sêmen no nitrogênio líquido por longos períodos de tempo também desempenha um papel importante nessa biotecnologia. Portanto, o objetivo desta revisão é descrever aspectos biotecnológicos, celulares e bioquímicos associados ao processo de criopreservação seminal em peixes de água doce, destacando os avanços, limitações e perspectivas.
RESUMO
Embryonic morphofunctional competence features regulating post-cryopreservation resumption of development are still poorly understood. In this study, we investigated the correlation between embryonic viability and the speed and ability to resume post-cryopreservation development. Thus, in vitro produced blastocysts were vitrified by the Cryotop method using standard protocols. Subsequently, the embryos were warmed, re-cultured, and classified into groups according to their speed and ability to resume post-cryopreservation development: embryos not re-expanded at 12h (NE12); embryos re-expanded at 12h and hatched at 24h (E12H24); embryos re-expanded at 12h and hatched at 48h (E12H48); embryos re-expanded at 12h and not hatched at 48h (E12NH48). Subsequently, the embryos were subjected to monitoring of total cell number and apoptosis. We identified that the blastocoel's ability to re-expand was negatively affected by the significant higher percentage of apoptotic cells observed in the NE12 group than in the other groups. A greater (P < 0.05) number of total cells, found in groups E12H24 and E12H48, seems to have a positive influence on the hatching capacity of blastocysts after cryopreservation. In conclusion, the total number of cells and apoptotic index correlated with the speed and ability to resume post-cryopreservation development. Apoptosis was a determinant for embryonic re-expansion, and the total cell number was crucial for blastocyst hatching.
Assuntos
Criopreservação , Vitrificação , Animais , Apoptose , Blastocisto , Criopreservação/veterinária , Desenvolvimento Embrionário , Feminino , GravidezRESUMO
This research aims to verify the influence of sulfated polysaccharides, extracted from the skin of tilapia, on the after thawing motility and morphology of P. brevis sperm. For this, 17 males were hormonally induced to reproduce, through the application of two doses of pituitary carp extract, 0.4 and 4.0mg kg-1. After the seminal collection, objective analyzes were performed and samples with motility greater than 80% were selected to form the pools. Then, the pools were frozen in solution supplemented, or not, with different concentrations of glycosaminoglycans (GAGs): 0 (control); 0.5; 1.0; 1.5; 2.0; 2.5; 3.0; 3.5; 4.0; 4.5 or 5.0mg mL-¹ (total of 10 treatments). The samples were placed in 0.25 mL French straws and submitted to an equilibrium time of 10 minutes at 4 ºC. Then, they were kept in the dry shipper for 15 minutes and finally stored in liquid nitrogen. After 15 days, samples were thawed in a water bath at 30 ºC for 16 seconds and evaluated for sperm motility and morphology. Thus, it was observed that the increase in GAGs caused a decrease in sperm motility, however the control and the concentration of 0.5mg mL-¹ presented very similar data. On the other hand, no decrease in normal sperm was observed with an increase in the concentration of GAGs. Therefore, it is concluded that the lowest concentration of GAGs is the most adequate to supplement the sperm freezing medium.(AU)
Assuntos
Animais , Masculino , Sêmen/efeitos dos fármacos , Sêmen/citologia , Motilidade dos Espermatozoides/efeitos dos fármacos , Glicosaminoglicanos/administração & dosagem , Glicosaminoglicanos/efeitos adversos , PeixesRESUMO
This research aims to verify the influence of sulfated polysaccharides, extracted from the skin of tilapia, on the after thawing motility and morphology of P. brevis sperm. For this, 17 males were hormonally induced to reproduce, through the application of two doses of pituitary carp extract, 0.4 and 4.0mg kg-1. After the seminal collection, objective analyzes were performed and samples with motility greater than 80% were selected to form the pools. Then, the pools were frozen in solution supplemented, or not, with different concentrations of glycosaminoglycans (GAGs): 0 (control); 0.5; 1.0; 1.5; 2.0; 2.5; 3.0; 3.5; 4.0; 4.5 or 5.0mg mL-¹ (total of 10 treatments). The samples were placed in 0.25 mL French straws and submitted to an equilibrium time of 10 minutes at 4 ºC. Then, they were kept in the dry shipper for 15 minutes and finally stored in liquid nitrogen. After 15 days, samples were thawed in a water bath at 30 ºC for 16 seconds and evaluated for sperm motility and morphology. Thus, it was observed that the increase in GAGs caused a decrease in sperm motility, however the control and the concentration of 0.5mg mL-¹ presented very similar data. On the other hand, no decrease in normal sperm was observed with an increase in the concentration of GAGs. Therefore, it is concluded that the lowest concentration of GAGs is the most adequate to supplement the sperm freezing medium.
Assuntos
Masculino , Animais , Glicosaminoglicanos/administração & dosagem , Glicosaminoglicanos/efeitos adversos , Motilidade dos Espermatozoides/efeitos dos fármacos , Peixes , Sêmen/citologia , Sêmen/efeitos dos fármacosRESUMO
Abstract Background: Cryopreservation preserves cellular viability under low temperatures, resulting in diminished intracellular enzymatic activity and reduced cellular metabolism that ultimately allows preserving genetic material for indefinite periods of time. Embryos submitted to cryopreservation suffer from considerable morphological and functional damage, resulting in reduced survival and development rates. Objective: To evaluate pregnancy and delivery rates of in vitro-produced (IVP) Nellore (Bos indicus) embryos after vitrification under field conditions. Methods: The IVP embryos at blastocyst (Bl) and expanded blastocyst (Bx) were transferred fresh (n= 137) or after vitrification (n= 127). Results: Pregnancy rates at 35 d for fresh embryos were lower in Bl (41.6) than in Bx (60.9) (p<0.05). After vitrification, pregnancy rates were similar at 35 d between Bl (38.0) and Bx (47.6) (p>0.05). Pregnancy loss at 60 d were similar (p>0.05) for both fresh (Bl: 3.1 and Bx: 4.8) and vitrified embryos (Bl: 1.9 and Bx: 4.7). Delivery rates were similar between groups (p>0.05). Conclusion: Both pregnancy and delivery rates of Bos indicus IVP embryos vitrified under field conditions are indistinguishable from fresh embryos.
Resumen Antecedentes: La criopreservación se caracteriza por el mantenimiento de la viabilidad celular a bajas temperaturas, resultando en reducido metabolismo y actividad enzimática intracelular, lo que permite la preservación del material genético por períodos de tiempo indefinidos. Los embriones sometidos a ésta técnica sufren daños morfológicos y funcionales considerables, dando como resultado una sobrevivencia y tasas de desarrollo reducidas. Objetivo: Evaluar la tasa de preñez a partir de embriones Nelore (Bos indicus) producidos in vitro (IVP) después de la vitrificación bajo condiciones de campo. Métodos: Embriones IVP en los estadios de blastocisto (Bl) y blastocisto expandido (Bx) se transfirieron en fresco (n= 137) o después de la vitrificación (n= 127). Resultados: La tasa de preñez a los 35 d fue menor para los embriones transferidos en fresco en fase Bl (41,6) en relación con los Bx (60,9) (p<0,05). Después de la vitrificación, las tasas de preñez a los 35 d fueron similares entre Bl (38,0) y Bx (47,6) (p>0,05). Las pérdidas de preñez a los 60 d fueron similares (p>0,05) tanto para embriones en fresco en Bl (3,1) y Bx (4,8) como para los vitrificados (Bl: 1,9 y Bx: 4,7). Las tasas de nacimiento fueron similares entre los grupos (p>0,05). Conclusión: Las tasas de preñez y nacimiento de embriones IVP vitrificados de Nelore (Bos indicus) bajo condiciones de campo son semejantes a las de embriones en fresco.
Resumo Antecedentes: A criopreservação é caracterizada pela manutenção da viabilidade celular em baixas temperaturas, resultando em atividade enzimática intracelular e metabolismo celular reduzido, que permite a preservação do material genético por períodos indefinidos de tempo. Embriões submetidos à criopreservação sofrem danos morfológicos e funcionais consideráveis, resultando em sobrevivência reduzida e menores taxas de desenvolvimento. Objetivo: Avaliar a taxa de prenhez a partir de embriões Nelore (Bos indicus) produzidos in vitro (IVP) após a vitrificação sob condições de campo. Métodos: Embriões IVP nos estádios de blastocisto (Bl) e blastocisto expandido (Bx) foram transferidos a fresco (n= 137) ou depois da vitrificação (n= 127). Resultados: A taxa de prenhez aos 35 d foi menor para os embriões transferidos a fresco na fase de Bl (41,6), em relação aos Bx (60,9) (p<0,05). Apos a vitrificação, as taxas de prenhez foram semelhantes aos 35 d entre Bl (38,0) e Bx (47,6) (p>0,05). As perdas de prenhez aos 60 d foram semelhantes (p>0,05) tanto para embriões a fresco nos estádios de Bl (3,1) e Bx (4,8), e vitrificados em Bl (1,9) e Bx (4,7). As taxas de nascimentos foram semelhantes entre os grupos (p>0,05). Conclusão: As taxas de prenhez e nascimentos dos embriões IVP vitrificados de Nelore (Bos indicus) sob condições de campo é semelhante àquela dos embriões a fresco.
RESUMO
Semen biotechniques may impair sperm quality due to excessive production of reactive oxygen species (ROS). Additionally, products of the oxidative reaction, especially involving lipids (e.g., malondialdehyde - MDA), may be even more harmful to sperm. Carnosine, previously reported to be present in seminal plasma of several species, may be a key factor on sperm tolerance to biotechniques by counterattacking the deleterious influence of MDA. Therefore, the aim of this study was to measure the levels of carnosine present in equine seminal plasma and relate these findings with sperm function and oxidative status during cooling and cryopreservation. Thus, semen samples were collected from 40 stallions in duplicate (Nâ¯=â¯80) and then submitted to cooling and cryopreservation. Samples were then allocated into groups of high and low tolerance to refrigeration and cryopreservation (bad cooler and good cooler/bad freezer and good freezer, respectively), and in groups of different concentrations of carnosine (High, Medium-high, Medium-low and Low carnosine). Samples were evaluated for sperm kinetics patterns, function of sperm structures and oxidative status. In good cooler samples, it was observed higher concentrations of carnosine (Good cooler: 224.98⯱â¯19.16â¯ng/mL; Bad cooler: 159.72⯱â¯15.99â¯ng/mL; pâ¯=â¯0.0056), ROS production (Good cooler: 26.40⯱â¯18.33%; Bad cooler: 18.33⯱â¯1.84%; pâ¯=â¯0.001) and lipid peroxidation rates (Good cooler: 193.23⯱â¯18.22â¯ng/mL; Bad cooler: 131.92⯱â¯12.25; pâ¯=â¯0.0064). Groups of samples with higher carnosine concentrations had lower levels of malondialdehyde (High: 79.33⯱â¯6.72â¯ng/mL; Medium-high: 140.45⯱â¯11.70â¯ng/mL; Medium-low: 202.57⯱â¯16.30â¯ng/mL and Low: 231.02⯱â¯32.35â¯ng/mL; pâ¯<â¯0.05), demonstrating that carnosine was effective in removing lipid peroxidation products. Due to the removal of seminal plasma during the cryopreservation process, no differences occurred in carnosine levels between bad and good freezer groups. In this context, this study provides relevant data for future therapies using carnosine during cryopreservation, aiming to replace the levels lost due to the necessary removal of seminal plasma.
Assuntos
Carnosina/química , Cavalos , Malondialdeído/química , Preservação do Sêmen/veterinária , Sêmen/química , Animais , Antioxidantes/química , Antioxidantes/farmacologia , Carnosina/farmacologia , Criopreservação/veterinária , Peroxidação de Lipídeos , MasculinoRESUMO
This is the first study of the highest elevation cyanobacteria-dominated microbial mat yet described. The desiccated mat was sampled in 2010 from an ephemeral rock pool at 5500 m above sea level in the Cordillera Vilcanota of southern Perú. After being frozen for 6 years at -20 °C in the lab, pieces of the mat were sequenced to fully characterize both the 16 and 18S microbial communities and experiments were conducted to determine if organisms in the mat could revive and become active under the extreme freeze-thaw conditions that these mats experience in the field. Sequencing revealed an unexpectedly diverse, multi-trophic microbial community with 16S OTU richness comparable to similar, seasonally desiccated mats from the Dry Valleys of Antarctica and low elevation sites in the Atacama Desert region. The bacterial community of the mat was dominated by phototrophs in the Cyanobacteria (Nostoc) and the Rhodospirillales, whereas the eukaryotic community was dominated by predators such as bdelloid rotifers (Philodinidae). Microcosm experiments showed that bdelloid rotifers in the mat were able to come out of dormancy and actively forage even under realistic field conditions (diurnal temperature fluctuations of -12 °C at night to + 27 °C during the day), and after being frozen for 6 years. Our results broaden our understanding of the diversity of life in periodically desiccated, high-elevation habitats and demonstrate that extreme freeze-thaw cycles per se are not a major factor limiting the development of at least some members of these unique microbial mat systems.
Assuntos
Biodiversidade , Cianobactérias/isolamento & purificação , Camada de Gelo/microbiologia , Rhodospirillales/isolamento & purificação , Rotíferos/isolamento & purificação , Altitude , Animais , Cianobactérias/genética , Dessecação , Ambientes Extremos , Congelamento , Peru , RNA Ribossômico 16S/genética , RNA Ribossômico 18S/genética , Rhodospirillales/genética , Rotíferos/genéticaRESUMO
Sperm vitrification is a cryopreservation method based on high-speed freezing by direct exposure of cells in liquid nitrogen (N2L), thereby avoiding the traditional cooling curves of freezing. The objective of this work was to determine the optimal warming temperature for vitrified human spermatozoa in order to maintain their fertilisation potential. Spermatozoa were cryopreserved by direct plunging into N2L and warmed at different temperatures for 5 and 10 s at 38, 40 and 42 °C. Sperm motility was evaluated by the CASA system and the sperm membrane function by HOST test. It was detected that progressive motility of sperm warmed at 38, 40 and 42 °C was 26.4 ± 8.4%; 56.6 ± 16.3% and 65.4 ± 15%, respectively, with statistically significant differences between the temperatures of 38 and 40 °C and 38 and 42 °C (P < 0.05). The plasma membrane function evaluated by HOST test was better preserved at 42 °C (76.3 ± 2.0%) compared to 40 °C (43 ± 2%) and 38 °C (65.6 ± 1.5%). The temperature in the thawing process can affect the motility and plasma membrane integrity and function. The warming at 42 °C for thawed vitrified sperm is the optimum temperature to preserve the sperm physiological parameters.
Assuntos
Criopreservação , Temperatura Alta , Preservação do Sêmen , Motilidade dos Espermatozoides , Espermatozoides , Humanos , Masculino , VitrificaçãoRESUMO
The aim of this study was to evaluate the pregnancy rate of in vitro produced embryos of Gyr cattle (Bos indicus) after cryopreservation by the vitrification method under field conditions. Blastocysts in different developmental stages were transferred to recipient cows either fresh (n = 140) or warmed after vitrification (n = 138). The pregnancy rates obtained for fresh embryos were 46.15% (initial blastocyst), 46.93% (blastocyst) and 50.0% (expanded blastocyst) at 35 days post-fertilization, and 43.58% (initial blastocyst), 46.93% (blastocyst) and 50.0% (expanded blastocyst) at 60 days. The pregnancy rates after embryo vitrification were 35.0% (initial blastocyst), 42.30% (blastocyst) and 43.47% (expanded blastocyst) at 35 days post-fertilization, and 32.50% (initial blastocyst), 38.46% (blastocyst) and 43.47% (expanded blastocyst) at 60 days. Embryo vitrification or blastocyst developmental stage did not affect pregnancy rates or incidence of embryonic death. In conclusion, vitrification of Gyr (Bos indicus) embryos under field conditions is an efficient method that can be implemented to use surplus in vitro produced embryos without affecting pregnancy rates...(AU)
Objetivou-se com o trabalho avaliar a taxa de prenhez a partir de embriões de bovinos da raça Gir (Bos indicus) produzidos in vitro após criopreservação em condições de campo pelo método de vitrificação. Blastocistos em diferentes estádios de desenvolvimento foram transferidos a fresco (n = 140) ou aquecidos após a vitrificação (n = 138). As taxas de prenhez de embriões frescos foram 46,15% (blastocisto inicial), 46,93% (blastocisto) e 50,00% (blastocisto expandido) aos 35 dias e 43,58% (blastocisto inicial), 46,93% (blastocisto) e 50,00% (blastocisto expandido) aos 60 dias pós-fertilização, respectivamente. As taxas de prenhez após a vitrificação foram 35,00% (blastocisto inicial), 42,30% (blastocisto) e 43,47% (blastocisto expandido) aos 35 dias e 32,50% (blastocisto inicial), 38,46% (blastocisto) e 43,47% (blastocisto expandido) aos 60 dias pós-fertilização, respectivamente. A vitrificação do embrião ou estádio do desenvolvimento não afetaram as taxas de prenhez ou incidência de morte embrionária. Em conclusão, a vitrificação de embriões de bovinos da raça Gir (Bos indicus) sob condições de campo é um método eficiente que pode ser implementado para aproveitar os embriões produzidos in vitro excedentes sem afetar a taxa de prenhez...(AU)
Assuntos
Animais , Bovinos , Prenhez , Embrião de Mamíferos , Vitrificação , Bovinos/classificaçãoRESUMO
The aim of this study was to evaluate the pregnancy rate of in vitro produced embryos of Gyr cattle (Bos indicus) after cryopreservation by the vitrification method under field conditions. Blastocysts in different developmental stages were transferred to recipient cows either fresh (n = 140) or warmed after vitrification (n = 138). The pregnancy rates obtained for fresh embryos were 46.15% (initial blastocyst), 46.93% (blastocyst) and 50.0% (expanded blastocyst) at 35 days post-fertilization, and 43.58% (initial blastocyst), 46.93% (blastocyst) and 50.0% (expanded blastocyst) at 60 days. The pregnancy rates after embryo vitrification were 35.0% (initial blastocyst), 42.30% (blastocyst) and 43.47% (expanded blastocyst) at 35 days post-fertilization, and 32.50% (initial blastocyst), 38.46% (blastocyst) and 43.47% (expanded blastocyst) at 60 days. Embryo vitrification or blastocyst developmental stage did not affect pregnancy rates or incidence of embryonic death. In conclusion, vitrification of Gyr (Bos indicus) embryos under field conditions is an efficient method that can be implemented to use surplus in vitro produced embryos without affecting pregnancy rates...
Objetivou-se com o trabalho avaliar a taxa de prenhez a partir de embriões de bovinos da raça Gir (Bos indicus) produzidos in vitro após criopreservação em condições de campo pelo método de vitrificação. Blastocistos em diferentes estádios de desenvolvimento foram transferidos a fresco (n = 140) ou aquecidos após a vitrificação (n = 138). As taxas de prenhez de embriões frescos foram 46,15% (blastocisto inicial), 46,93% (blastocisto) e 50,00% (blastocisto expandido) aos 35 dias e 43,58% (blastocisto inicial), 46,93% (blastocisto) e 50,00% (blastocisto expandido) aos 60 dias pós-fertilização, respectivamente. As taxas de prenhez após a vitrificação foram 35,00% (blastocisto inicial), 42,30% (blastocisto) e 43,47% (blastocisto expandido) aos 35 dias e 32,50% (blastocisto inicial), 38,46% (blastocisto) e 43,47% (blastocisto expandido) aos 60 dias pós-fertilização, respectivamente. A vitrificação do embrião ou estádio do desenvolvimento não afetaram as taxas de prenhez ou incidência de morte embrionária. Em conclusão, a vitrificação de embriões de bovinos da raça Gir (Bos indicus) sob condições de campo é um método eficiente que pode ser implementado para aproveitar os embriões produzidos in vitro excedentes sem afetar a taxa de prenhez...
Assuntos
Animais , Bovinos , Bovinos/classificação , Embrião de Mamíferos , Prenhez , VitrificaçãoRESUMO
The study was conducted with the objective of comparing the toxicity and the effect of the combination of intra and extracellular cryoprotectants in curimba Prochilodus lineatus sperm cells subjected to cryopreservation. Semen from 19 males were analyzed and diluted in four solutions comprise of intra and extracellular cryoprotectants in the following combinations: methanol+lactose, methanol+egg yolk, DMSO+lactose and DMSO+egg yolk. A portion of the diluted semen was frozen while the remaining fraction was kept in repose and evaluated after 10 min. For freezing, the diluted samples were packaged in 0.50 mL straws and placed into liquid nitrogen vapor for 24 h and, after this time, submerged into liquid nitrogen for 10 days. The combination of DMSO+lactose was less toxic to the diluted semen, resulting in higher motility rates and durations when compared to the other treatments. After thawing, the highest motility rate and duration were obtained using lactose as extracellular cryoprotectant, regardless of its combination. There was no significant difference between treatments when analyzing sperm morphology after thawing. Considering the effects of the tested treatments, the use of lactose as an extracellularcryoprotectant added with DMSO or methanol is the most suitable, since these combinations presented the highest motility rates and durations and low morphological change rate after thawing.(AU)
O estudo foi realizado com o objetivo de comparar a toxicidade e o efeito da combinação de crioprotetoresintra e extracelulares em espermatozóides de curimba Prochilodus lineatus submetidos à criopreservação. O sêmen de 19 machos foi analisado e diluído em quatro soluções com crioprotetores intra e extracelulares nas seguintes combinações: metanol+lactose, metanol+gema de ovo, DMSO+lactose e DMSO+gema de ovo. Uma porção do sêmen diluído foi congelada enquanto que a fração remanescente foi mantida em repouso e avaliada após 10 min. Para o congelamento, as amostras diluídas foram envasadas em palhetas de 0,50 mL e colocadas em vapor de nitrogênio líquido durante 24 h e, após este tempo, submersas em nitrogênio líquido durante 10 dias. A combinação de DMSO+lactose se mostrou menos tóxica para o sêmen diluído, resultando em taxas mais elevadas de motilidade e duração espermática quando comparadas com os outros tratamentos. Após descongelamento, as maiores taxas de motilidade e duração foram obtidas usando lactose como crioprotector extracelular, independentemente da sua combinação. Não houve diferença significativa entre os tratamentos ao analisar a morfologia espermática após a descongemento. Considerando-se os efeitos dos tratamentos utilizados, o uso de lactose como crioprotector extracelular, adicionada ao DMSO ou metanol, é o mais adequado, uma vez que estascombinações apresentaram maiores taxas de motilidade e duração espermática, e baixa taxa de alteração morfológica após o descongelamento.(AU)
Assuntos
Animais , Preservação do Sêmen/veterinária , Preservação do Sêmen/métodos , Crioprotetores/análise , Análise do Sêmen , Lactose/análise , Metanol/análise , Caraciformes , Criopreservação/veterinária , Criopreservação/métodosRESUMO
The study was conducted with the objective of comparing the toxicity and the effect of the combination of intra and extracellular cryoprotectants in curimba Prochilodus lineatus sperm cells subjected to cryopreservation. Semen from 19 males were analyzed and diluted in four solutions comprise of intra and extracellular cryoprotectants in the following combinations: methanol+lactose, methanol+egg yolk, DMSO+lactose and DMSO+egg yolk. A portion of the diluted semen was frozen while the remaining fraction was kept in repose and evaluated after 10 min. For freezing, the diluted samples were packaged in 0.50 mL straws and placed into liquid nitrogen vapor for 24 h and, after this time, submerged into liquid nitrogen for 10 days. The combination of DMSO+lactose was less toxic to the diluted semen, resulting in higher motility rates and durations when compared to the other treatments. After thawing, the highest motility rate and duration were obtained using lactose as extracellular cryoprotectant, regardless of its combination. There was no significant difference between treatments when analyzing sperm morphology after thawing. Considering the effects of the tested treatments, the use of lactose as an extracellularcryoprotectant added with DMSO or methanol is the most suitable, since these combinations presented the highest motility rates and durations and low morphological change rate after thawing.
O estudo foi realizado com o objetivo de comparar a toxicidade e o efeito da combinação de crioprotetoresintra e extracelulares em espermatozóides de curimba Prochilodus lineatus submetidos à criopreservação. O sêmen de 19 machos foi analisado e diluído em quatro soluções com crioprotetores intra e extracelulares nas seguintes combinações: metanol+lactose, metanol+gema de ovo, DMSO+lactose e DMSO+gema de ovo. Uma porção do sêmen diluído foi congelada enquanto que a fração remanescente foi mantida em repouso e avaliada após 10 min. Para o congelamento, as amostras diluídas foram envasadas em palhetas de 0,50 mL e colocadas em vapor de nitrogênio líquido durante 24 h e, após este tempo, submersas em nitrogênio líquido durante 10 dias. A combinação de DMSO+lactose se mostrou menos tóxica para o sêmen diluído, resultando em taxas mais elevadas de motilidade e duração espermática quando comparadas com os outros tratamentos. Após descongelamento, as maiores taxas de motilidade e duração foram obtidas usando lactose como crioprotector extracelular, independentemente da sua combinação. Não houve diferença significativa entre os tratamentos ao analisar a morfologia espermática após a descongemento. Considerando-se os efeitos dos tratamentos utilizados, o uso de lactose como crioprotector extracelular, adicionada ao DMSO ou metanol, é o mais adequado, uma vez que estascombinações apresentaram maiores taxas de motilidade e duração espermática, e baixa taxa de alteração morfológica após o descongelamento.
Assuntos
Animais , Análise do Sêmen , Caraciformes , Crioprotetores/análise , Lactose/análise , Metanol/análise , Preservação do Sêmen/métodos , Preservação do Sêmen/veterinária , Criopreservação/métodos , Criopreservação/veterináriaRESUMO
Background: cryopreservation is an important biotechnological tool in the conservation of biodiversity, particularly for endangered species. Objective: to evaluate six different spermatozoa/oocyte ratios using fresh and cryopreserved semen in bocachico fish (Prochilodus magdalenae). Methods: fresh semen was collected and its quality determined to verify cryopreservation feasibility. The semen was put in 5 mL straws and mixed with a solution (5.5% glucose, 12% egg yolk, and 10% dimethyl sulfoxide -DMSO-) in a 1:4 dilution (semen:solution). The semen was frozen in nitrogen vapor dry shipper for 30 min, rapidly transferred to storage thermos, and submerged directly into liquid nitrogen (LN; -196 °C). Straws were thawed at 60 ºC for 45 seconds. Motility, velocity, and sperm progressivity of fresh and cryopreserved semen were assessed using Sperm Class Analyzer (SCA®) software. Each proportion of spermatozoa/oocyte was assessed with 2 g of eggs (1,630 ± 87 eggs/g) to evaluate fertility (F), hatching (H), and larval survival (LS) rates. Results: the best reproductive performance for fresh semen was obtained inseminating with 160,000 spermatozoa/oocyte (F = 75.0%, H = 67.7%, LS = 32.7%). Similarly, the best reproductive performance for cryopreserved semen was achieved with 320,000 spermatozoa/oocyte (F = 70.0%, H = 48.6%, LS = 19.5%). Conclusion: it is possible to achieve adequate reproductive performance in bocachico fish using cryopreserved sperm (10% DMSO, 5.5% glucose, and 12% egg yolk) at twice the spermatozoa/oocyte ratio used with fresh semen.
Antecedentes: la crioconservación es una herramienta biotecnológica importante para la conservación de la biodiversidad, particularmente de especies en peligro. Objetivo: evaluar seis proporciones diferentes entre espermatozoides/ovocito en la fertilización de bocachico (Prochilodus magdalenae), usando semen fresco o crioconservado. Métodos: se colectó semen y se determinó su calidad para verificar su viabilidad de crioconservación. El semen fue colocado en pajillas de 5 mL y mezclado con una solución crioconservante (5,5% glucosa, 12% yema de huevo y 10% dimethyl sulfoxido -DMSO-) en una dilución 1:4 (semen:solución). El semen fue congelado en un termo de vapores de nitrógeno por 30 min y rápidamente se transfirió a termos de almacenamiento sumergiéndolo directamente en nitrógeno líquido (LN; -196 °C). Las pajillas fueron descongeladas a 60 ºC por 45 segundos. La motilidad, velocidad y progresividad de los espermatozoides, tanto de semen fresco como del congelado, fueron evaluadas usando el software Sperm Class Analyzer (SCA®). Cada proporción de espermatozoides/ovocito fue evaluada en 2 g de huevos (1.630 ± 87 huevos/g) para evaluar fertilidad (F), eclosión (H) y sobrevivencia larval (LS). Resultados: el mejor desempeño reproductivo con semen fresco fue obtenido inseminando con la proporción de 160.000 espermatozoides/ovocito (F = 75,0%, H = 67,7%, LS = 32,7%). De manera similar, el mejor desempeño reproductivo con semen crioconservado fue logrado con la proporción de 320.000 espermatozoide/ovocito (F = 70,0%, H = 48,6%, LS = 19,5%). Conclusión: es posible lograr un adecuado desempeño reproductivo en bocachico usando semen crioconservado (10% DMSO, 5,5% glucosa y 12% yema de huevo) cuando la relación espermatozoide/ovocito usada es del doble de la proporción aplicada para semen fresco.
Antecedentes: a criopreservação é uma ferramenta biotecnológica importante na conservação da biodiversidade, particularmente de espécies ameaçadas. Objetivo: foram avaliadas seis proporções de espermatozoides/ovócito na fertilização usando sêmen fresco e crioconservado em fertilização de bocachico (Prochilodus magdalenae), Métodos: o sêmen fresco foi coletado e determinada sua qualidade para verificar a viabilidade de crioconservação. O sêmen foi colocado em palhetas de 5 mL e misturado com a solução crioconservante (5,5% glicose, 12% gema de ovo e 10% dimetilsulfóxido -DMSO-) em numa diluição 1:4 (sêmen:solução). O sêmen foi congelado em botijão de vapores de nitrogênio por 30 min e rapidamente transferido a botijão de armazenagem submergindo-os diretamente em nitrogênio líquido (LN; -196 °C). As palhetas foram descongeladas a 60 ºC por 45 segundos. A motilidade, velocidade e progressividade dos espermatozoides, tanto de sêmen fresco quanto de congelado, foram avaliadas usando o software Sperm Class Analyzer (SCA®). Para avaliar fertilidade (F), eclosão (H) e sobrevivência larval (LS), cada relação de espermatozóide/oócito foi avaliada em 2 g de oócitos (1.630 ± 87 ovos/g). Resultados: o melhor desempenho reprodutivo com sêmen fresco foi obtido inseminando com proporção 160.000 espermatozoides/oócito (F = 75,0%, H = 67,7%, LS = 32,7%). O melhor desempenho reprodutivo com sêmen crioconservado foi verificado na proporção de 320.000 espermatozoides/oócito (F = 70,0%, H = 48,6%, LS = 19,5%). Conclusão: é possível alcançar um adequado desempenho reprodutivo em bocachico usando sêmen crioconservado (10% DMSO, 5,5% glicose e 12% gema de ovo) quando a proporção espermatozoide/oócito usada é o dobro da utilizada para sêmen fresco.
RESUMO
The experiment aimed to compare conventional freezing and different vitrification protocols for cryopreservation of caprine embryos at morphological, ultrastructural, and functional levels. Caprine embryos produced in vivo were allocated randomly to three groups: (1) conventional freezing with ethylene glycol (EG); (2) dimethyl sulfoxide + EG (DMSO/EG) vitrification; and (3) dimethylformamide + EG (DMF/EG) vitrification. All groups were scored for cell viability (propidium iodide staining and ultrastructural levels) and re-expansion rate after thawing or warming. Embryos subjected to DMSO/EG vitrification showed higher cell viability (73.33%), compared with DMF/EG vitrification and conventional freezing group embryos (40.00 and 66.66%, respectively). The ultrastructural study revealed that vitrified embryos had greater preservation of cellular structure than embryos from conventional freezing with EG. DMSO/EG vitrification resulted in higher rates of re-expansion in vitro (47.36%) than DMF/EG vitrification (31.58%), and conventional freezing (25.00%). In conclusion, caprine embryos produced in vivo are better cryopreserved after vitrification than conventional freezing, therefore we conclude that DMSO/EG vitrification is the most effective protocol for cryopreservation.
Assuntos
Blastocisto/fisiologia , Criopreservação/métodos , Embrião de Mamíferos/fisiologia , Cabras , Animais , Blastocisto/ultraestrutura , Crioprotetores , Dimetil Sulfóxido , Dimetilformamida , Embrião de Mamíferos/citologia , Embrião de Mamíferos/ultraestrutura , Etilenoglicol , Feminino , Congelamento , Masculino , Gravidez , VitrificaçãoRESUMO
Modern livestock breeding is basically dependent on the proper use of semen for artificial insemination (AU) of femeles and of other reproductive biotechnologies such as the production of embryos in vitro for embryo transfer (IVP). Both these techniques have made possible not only the wide dissemmation of genetic material onto breeding populations but also anhanced the selection of best sires, owing to the development of better diagnostic techniques for sperm function and of preservation of seminal material over time. Although use ofliquid semen cooled to room temperature, to intermediate temperatures (+16-20ºC) or chilled (+5ºC) dominates in different species cryopreservation is preferred in bovine A1 and it is advancing in other species by the design of new containers, freezing methods and the use of better insemination strategies. Techniques to separate the aliquot of most robust spermatozoa from an ejaculate have shown a renascent particularly for sires with low sperm quality, and technological advances in separating spermatozoa for c hromosomal sex make the technique suitable for commercial use, following applicat ion of novel findings in sperm and seminal plasma (SP) diagnostics and function. Alongside, knowledge of the epigenome and signalling c apabilities of the semen (sperm and SP) call s for further studies regarding transgene production via ICSI for IVP or AI.(AU)