Effect of catalase, superoxide dismutase and reduced glutathione in LDL extender on ovine cryopreserved sperm viability

Paola Pereira das Neves Snoeck; Luís Cláudio Oliveira Moura; Carlos Augusto Alanis Clemente; Ana Maria Loaiza-Echeverri; Mariana Machado Neves; Ivan Bezerra Allaman; Marc Henry

doi:10.5433/1679-0359.2015v36n4p2593

Semina: Ciências Agrárias (Aug 2015)

Effect of catalase, superoxide dismutase and reduced glutathione in LDL extender on ovine cryopreserved sperm viability

Paola Pereira das Neves Snoeck ,
Luís Cláudio Oliveira Moura ,
Carlos Augusto Alanis Clemente ,
Ana Maria Loaiza-Echeverri ,
Mariana Machado Neves ,
Ivan Bezerra Allaman ,
Marc Henry

Affiliations

Paola Pereira das Neves Snoeck: Universidade Estadual de Santa Cruz
Luís Cláudio Oliveira Moura: Universidade Estadual de Santa Cruz
Carlos Augusto Alanis Clemente: Universidade Federal de Minas Gerais
Ana Maria Loaiza-Echeverri: Universidade Federal de Minas Gerais
Mariana Machado Neves: Universidade Federal de Viçosa
Ivan Bezerra Allaman: Universidade Estadual de Santa Cruz
Marc Henry: Universidade Federal de Minas Gerais

DOI: https://doi.org/10.5433/1679-0359.2015v36n4p2593
Journal volume & issue: Vol. 36, no. 4
pp. 2593 – 2602

Abstract

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The aim of this study was to evaluate the motility, kinetics and membrane integrity of ovine sperm cryopreserved in extenders containing 8% LDL with enzymatic antioxidants at different concentrations. Four Santa Inês rams were used to form four pools of semen (each pool containing ejaculates from four ram, totaling four ejaculates per animal). Each seminal pool was divided into eight aliquots for the following treatments: 1) Tris-glucose-glycerol (TGG) + (16%) egg yolk (control 1); 2) TGG + 8% (w/v) LDL (control 2); 3) TGG + 8% LDL + catalase 100 U/mL; 4) TGG + 8% LDL + catalase 200 U/mL; 5) TGG + 8% LDL + superoxide dismutase 100 U/mL; 6) TGG + 8% LDL + superoxide dismutase 200 U/mL; 7) TGG + 8% LDL + reduced glutathione 5 mM; and 8) TGG + 8% LDL + reduced glutathione 10 mM. The samples were packed into 0.25 mL straws, cooled (-0.25 °C/ min), maintained at 5 °C for 2 h and then frozen (-25 °C/ min) using a TK4000®. Immediately after thawing (38 °C/ 30 s), sperm motility and movement characteristics were assessed by computer sperm analysis (CASA). The structural integrity of the plasma and acrosomal membranes was analyzed using fluorescent dyes. The functional integrity of membranes was assessed using a hypoosmotic swelling test. As assessed by ANOVA, significant differences (P<0.05) among treatments were only observed for VCL, VSL and VAP. For the VCL variable, the 2, 3, 4, 5, 6 and 7 extenders were similar and higher than 1 and 8 extenders, the latter being similar to each other. For the VSL variable, the 3, 4, 5, 6 and 7 extenders were similar and higher than 1, 2 and 8 extenders, the latter being similar to each other. For the VAP variable, the 3, 4 and 6 extenders were similar and higher than 1, 2, 5, 7 and 8 extenders, the latter being similar to each other. In conclusion, enzymatic antioxidants as catalase e superoxide dismutase improve the protective activity of extenders containing LDL on frozen ovine sperm.

Cryopreservation; Semen; Enzymatic antioxidants; Santa Inês

Published in Semina: Ciências Agrárias

ISSN: 1676-546X (Print); 1679-0359 (Online)
Publisher: Universidade Estadual de Londrina
Country of publisher: Brazil
LCC subjects: Agriculture: Agriculture (General)
Website: https://www.uel.br/revistas/uel/index.php/semagrarias/index

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