Efeito de antioxidantes aos espermatozoides de equinos submetidos ao estresse térmico

Detalhes bibliográficos
Autor(a) principal: OLIVEIRA, Aline França Dias
Data de Publicação: 2010
Tipo de documento: Dissertação
Idioma: por
Título da fonte: Repositório Institucional da UFG
dARK ID: ark:/38995/0013000002m6d
Texto Completo: http://repositorio.bc.ufg.br/tede/handle/tde/1256
Resumo: The evaluation of the reproductive capacity of stallions and semen cooled and / or frozen is of fundamental importance in practical breeding of horses. Whereas predicting the fertility of a stallion is still a subjective decision, the present study was conducted to evaluate different staining techniques, as well as tests that assess the viability of semen in horses, studying the effects of the addition of cysteine and glutathione in plasma membrane integrity of sperm DNA, and to evaluate the effects of the addition of these antioxidants in preserving the viability of sperm undergoing incubation and refrigerated for short periods. We used semen from six stallions, wich were split into seven samples, one kept as control (Control Group) and other antioxidants cysteine was added at a ratio of 1.0 mM (Group C1, 0), 1.5 mM (Group C1, 5), 2.5 mM (Group C 2.5) and glutathione also at 1.0 mM (Group G1, 0), 1.5 mM (Group G1, 5) and 2.5 mM (Group G 2.5 ). All tests were performed every six hours. The three treatments were: Treatment I cooled to 12 &#8304;C for 12 hours (zero hour; 6h resf.; 12h resf.) Chilled in boxes; Treatment II incubated in a water bath at 37 &#8304;C for 12 hours (6h 37 ° C, 12h 37 ° C) and Treatment III - cooled and subsequently incubated, according to the treatments I and II. The evaluation of plasma membrane integrity was performed by staining eosine-nigrosin; acrosomal membrane by FITC-PSA and DNA by acridine orange. For each analysis were numbered 200 to 500 cells. The evaluation of the viability of sperm was performed by MTT assay according to Mosmann (1983). The results showed that antioxidants were effective (p <0.05) in keeping the DNA intact chromatin, especially glutathione. In the acrosome of antioxidants were protective, at times 18 and 24 hours, and in other treatments, no significant difference (p> 0.05) between control and treated groups. The MTT test showed that groups treated with antioxidants had absorbance values similar to those of control, showing positive effect (p <0.05) only when cooled by six o'clock in the cysteine group 2.5. In relation to the plasma membrane of spermatozoa stained with eosin-nigrosin, no protective effect of antioxidants in the samples. The values of their averages were close to the control group (p> 0.05). One factor was estimated that cooling per se, independent of the addition of antioxidants used, has been effective in protecting the sperm. And the incubation at 37 &#8304; C causes these cells, and the addition of cysteine and glutathione were efficient, if not protect, but to maintain the integrity of the factors evaluated, not causing more damage to sperm.
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spelling GUILLO, Lídia Andreuhttp://lattes.cnpq.br/3401436781775091http://lattes.cnpq.br/9830889124120940OLIVEIRA, Aline França Dias2014-07-29T15:16:30Z2011-06-222010-10-05OLIVEIRA, Aline França Dias. Effect of antioxidants on stallion spermatozoa under heat stress. 2010. 76 f. Dissertação (Mestrado em Ciências Biolóicas) - Universidade Federal de Goiás, Goiânia, 2010.http://repositorio.bc.ufg.br/tede/handle/tde/1256ark:/38995/0013000002m6dThe evaluation of the reproductive capacity of stallions and semen cooled and / or frozen is of fundamental importance in practical breeding of horses. Whereas predicting the fertility of a stallion is still a subjective decision, the present study was conducted to evaluate different staining techniques, as well as tests that assess the viability of semen in horses, studying the effects of the addition of cysteine and glutathione in plasma membrane integrity of sperm DNA, and to evaluate the effects of the addition of these antioxidants in preserving the viability of sperm undergoing incubation and refrigerated for short periods. We used semen from six stallions, wich were split into seven samples, one kept as control (Control Group) and other antioxidants cysteine was added at a ratio of 1.0 mM (Group C1, 0), 1.5 mM (Group C1, 5), 2.5 mM (Group C 2.5) and glutathione also at 1.0 mM (Group G1, 0), 1.5 mM (Group G1, 5) and 2.5 mM (Group G 2.5 ). All tests were performed every six hours. The three treatments were: Treatment I cooled to 12 &#8304;C for 12 hours (zero hour; 6h resf.; 12h resf.) Chilled in boxes; Treatment II incubated in a water bath at 37 &#8304;C for 12 hours (6h 37 ° C, 12h 37 ° C) and Treatment III - cooled and subsequently incubated, according to the treatments I and II. The evaluation of plasma membrane integrity was performed by staining eosine-nigrosin; acrosomal membrane by FITC-PSA and DNA by acridine orange. For each analysis were numbered 200 to 500 cells. The evaluation of the viability of sperm was performed by MTT assay according to Mosmann (1983). The results showed that antioxidants were effective (p <0.05) in keeping the DNA intact chromatin, especially glutathione. In the acrosome of antioxidants were protective, at times 18 and 24 hours, and in other treatments, no significant difference (p> 0.05) between control and treated groups. The MTT test showed that groups treated with antioxidants had absorbance values similar to those of control, showing positive effect (p <0.05) only when cooled by six o'clock in the cysteine group 2.5. In relation to the plasma membrane of spermatozoa stained with eosin-nigrosin, no protective effect of antioxidants in the samples. The values of their averages were close to the control group (p> 0.05). One factor was estimated that cooling per se, independent of the addition of antioxidants used, has been effective in protecting the sperm. And the incubation at 37 &#8304; C causes these cells, and the addition of cysteine and glutathione were efficient, if not protect, but to maintain the integrity of the factors evaluated, not causing more damage to sperm.A avaliação da eficácia reprodutiva do garanhão e do sêmen resfriado e&#8260;ou congelado é de fundamental importância na prática reprodutiva dos eqüinos. Predizer a fertilidade de um garanhão constitui uma decisão subjetiva. O presente estudo foi realizado com o objetivo de testar diferentes técnicas de coloração, assim como testes que avaliem a viabilidade do sêmen de eqüinos, estudando os efeitos da adição de cisteína e glutationa na integridade da membrana plasmática, do DNA espermático, além de avaliar os efeitos da adição desses antioxidantes na preservação da viabilidade dos espermatozóides submetidos à incubação e refrigeração por curtos períodos. Foi utilizado sêmen de seis garanhões, que foram fracionados em sete amostras, sendo uma mantida como controle (Grupo Controle) e às outras foi adicionado os antioxidantes cisteína, na proporção de 1,0mM (Grupo C1,0); 1,5mM (Grupo C1,5); 2,5mM (Grupo C 2,5) e glutationa também na proporção de 1,0mM (Grupo G1,0); 1,5mM (Grupo G1,5) e 2,5mM (Grupo G 2,5). Todas as análises foram realizadas a cada seis horas. Os três tratamentos foram: Tratamento I resfriado a 12 °C, por 12 horas (zero hora; 6h resf.; 12h resf.), em caixas refrigeradas; Tratamento II incubado em banho-maria a 37 °C, por 12 horas (6h 37° C; 12h 37° C) e Tratamento III resfriado e posteriormente incubado, conforme os Tratamentos I e II. A avaliação da integridade da membrana plasmática foi feita pela coloração eosina-nigrosina; da membrana acrossomal pelo FITC-PSA e do DNA pela laranja de acridina. A avaliação da viabilidade do sêmen foi realizada pelo ensaio do MTT, de acordo com Mosmann(1983). Os resultados obtidos mostraram que os antioxidantes foram eficientes (p<0,05) em manter a cromatina do DNA intacta, especialmente a glutationa. Na membrana acrossomal houve proteção dos antioxidantes, nos momentos 18 e 24 horas, sendo que nos demais tratamentos, não houve diferença significativa (p>0,05) entre os grupos tratados e o grupo controle. O teste do MTT mostrou que os grupos tratados com antioxidantes tiveram valores de absorbância próximos aos do controle, mostrando efeito positivo (p<0,05) apenas quando resfriados por seis horas, no grupo cisteína 2,5. Em relação à membrana plasmática dos espermatozóides, corados por eosina-nigrosina, não houve efeito protetor dos antioxidantes nas amostras avaliadas. Um fator avaliado foi que o resfriamento, por si só, independente da adição dos antioxidantes utilizados, já foi eficaz em proteger os espermatozóides. E a incubação a 37&#8304; C causa danos a essas células, e a adição de cisteína e glutationa foi eficiente em, senão proteger, mas manter a integridade dos fatores avaliados, não causando mais danos aos espermatozóides.Made available in DSpace on 2014-07-29T15:16:30Z (GMT). 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dc.title.por.fl_str_mv Efeito de antioxidantes aos espermatozoides de equinos submetidos ao estresse térmico
dc.title.alternative.eng.fl_str_mv Effect of antioxidants on stallion spermatozoa under heat stress
title Efeito de antioxidantes aos espermatozoides de equinos submetidos ao estresse térmico
spellingShingle Efeito de antioxidantes aos espermatozoides de equinos submetidos ao estresse térmico
OLIVEIRA, Aline França Dias
cisteina
glutationa
MTT
FITC-PSA
laranja de acridina
espermatozóide
garanhão
cystein
glutathione
MTT
FITC-PSA
acridine orange
spermatozoa
stallion
CNPQ::CIENCIAS BIOLOGICAS::BIOQUIMICA::BIOLOGIA MOLECULAR
title_short Efeito de antioxidantes aos espermatozoides de equinos submetidos ao estresse térmico
title_full Efeito de antioxidantes aos espermatozoides de equinos submetidos ao estresse térmico
title_fullStr Efeito de antioxidantes aos espermatozoides de equinos submetidos ao estresse térmico
title_full_unstemmed Efeito de antioxidantes aos espermatozoides de equinos submetidos ao estresse térmico
title_sort Efeito de antioxidantes aos espermatozoides de equinos submetidos ao estresse térmico
author OLIVEIRA, Aline França Dias
author_facet OLIVEIRA, Aline França Dias
author_role author
dc.contributor.advisor1.fl_str_mv GUILLO, Lídia Andreu
dc.contributor.advisor1Lattes.fl_str_mv http://lattes.cnpq.br/3401436781775091
dc.contributor.authorLattes.fl_str_mv http://lattes.cnpq.br/9830889124120940
dc.contributor.author.fl_str_mv OLIVEIRA, Aline França Dias
contributor_str_mv GUILLO, Lídia Andreu
dc.subject.por.fl_str_mv cisteina
glutationa
MTT
FITC-PSA
laranja de acridina
espermatozóide
garanhão
topic cisteina
glutationa
MTT
FITC-PSA
laranja de acridina
espermatozóide
garanhão
cystein
glutathione
MTT
FITC-PSA
acridine orange
spermatozoa
stallion
CNPQ::CIENCIAS BIOLOGICAS::BIOQUIMICA::BIOLOGIA MOLECULAR
dc.subject.eng.fl_str_mv cystein
glutathione
MTT
FITC-PSA
acridine orange
spermatozoa
stallion
dc.subject.cnpq.fl_str_mv CNPQ::CIENCIAS BIOLOGICAS::BIOQUIMICA::BIOLOGIA MOLECULAR
description The evaluation of the reproductive capacity of stallions and semen cooled and / or frozen is of fundamental importance in practical breeding of horses. Whereas predicting the fertility of a stallion is still a subjective decision, the present study was conducted to evaluate different staining techniques, as well as tests that assess the viability of semen in horses, studying the effects of the addition of cysteine and glutathione in plasma membrane integrity of sperm DNA, and to evaluate the effects of the addition of these antioxidants in preserving the viability of sperm undergoing incubation and refrigerated for short periods. We used semen from six stallions, wich were split into seven samples, one kept as control (Control Group) and other antioxidants cysteine was added at a ratio of 1.0 mM (Group C1, 0), 1.5 mM (Group C1, 5), 2.5 mM (Group C 2.5) and glutathione also at 1.0 mM (Group G1, 0), 1.5 mM (Group G1, 5) and 2.5 mM (Group G 2.5 ). All tests were performed every six hours. The three treatments were: Treatment I cooled to 12 &#8304;C for 12 hours (zero hour; 6h resf.; 12h resf.) Chilled in boxes; Treatment II incubated in a water bath at 37 &#8304;C for 12 hours (6h 37 ° C, 12h 37 ° C) and Treatment III - cooled and subsequently incubated, according to the treatments I and II. The evaluation of plasma membrane integrity was performed by staining eosine-nigrosin; acrosomal membrane by FITC-PSA and DNA by acridine orange. For each analysis were numbered 200 to 500 cells. The evaluation of the viability of sperm was performed by MTT assay according to Mosmann (1983). The results showed that antioxidants were effective (p <0.05) in keeping the DNA intact chromatin, especially glutathione. In the acrosome of antioxidants were protective, at times 18 and 24 hours, and in other treatments, no significant difference (p> 0.05) between control and treated groups. The MTT test showed that groups treated with antioxidants had absorbance values similar to those of control, showing positive effect (p <0.05) only when cooled by six o'clock in the cysteine group 2.5. In relation to the plasma membrane of spermatozoa stained with eosin-nigrosin, no protective effect of antioxidants in the samples. The values of their averages were close to the control group (p> 0.05). One factor was estimated that cooling per se, independent of the addition of antioxidants used, has been effective in protecting the sperm. And the incubation at 37 &#8304; C causes these cells, and the addition of cysteine and glutathione were efficient, if not protect, but to maintain the integrity of the factors evaluated, not causing more damage to sperm.
publishDate 2010
dc.date.issued.fl_str_mv 2010-10-05
dc.date.available.fl_str_mv 2011-06-22
dc.date.accessioned.fl_str_mv 2014-07-29T15:16:30Z
dc.type.status.fl_str_mv info:eu-repo/semantics/publishedVersion
dc.type.driver.fl_str_mv info:eu-repo/semantics/masterThesis
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dc.identifier.citation.fl_str_mv OLIVEIRA, Aline França Dias. Effect of antioxidants on stallion spermatozoa under heat stress. 2010. 76 f. Dissertação (Mestrado em Ciências Biolóicas) - Universidade Federal de Goiás, Goiânia, 2010.
dc.identifier.uri.fl_str_mv http://repositorio.bc.ufg.br/tede/handle/tde/1256
dc.identifier.dark.fl_str_mv ark:/38995/0013000002m6d
identifier_str_mv OLIVEIRA, Aline França Dias. Effect of antioxidants on stallion spermatozoa under heat stress. 2010. 76 f. Dissertação (Mestrado em Ciências Biolóicas) - Universidade Federal de Goiás, Goiânia, 2010.
ark:/38995/0013000002m6d
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dc.publisher.department.fl_str_mv Ciências Biolóicas
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