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dc.contributor.author Lanes, Carlos Frederico Ceccon
dc.contributor.author Okamoto, Marcelo Hideo
dc.contributor.author Cavalcanti, Paulo Varoni
dc.contributor.author Collares, Tiago Veiras
dc.contributor.author Campos, Vinicius Farias
dc.contributor.author Deschamps, João Carlos
dc.contributor.author Robaldo, Ricardo Berteaux
dc.contributor.author Marins, Luis Fernando Fernandes
dc.contributor.author Sampaio, Luís André Nassr de
dc.date.accessioned 2012-12-11T16:27:41Z
dc.date.available 2012-12-11T16:27:41Z
dc.date.issued 2008
dc.identifier.citation LANES, Carlos Frederico Ceccon et al. Cryopreservation of brazilian flounder (paralichthys orbignyanus) sperm. Aquaculture, Amsterdam, v. 275, p. 361-365, 2008. Disponível em: <http://ac.els-cdn.com/S0044848608000033/1-s2.0-S0044848608000033-main.pdf?_tid=f0a42490-2dfe-11e2-bfc6-00000aacb35d&acdnat=1352858555_ea8c211de5207f9067f67a3e5e40ed44>. Acesso em 10 nov. 2012. pt_BR
dc.identifier.uri http://repositorio.furg.br/handle/1/2983
dc.description.abstract The Brazilian flounder, Paralichthys orbignyanus, is being considered for aquaculture due to its high demand and market price. Reproduction and larviculture studies have demonstrated the feasibility of massive fingerling production, and techniques that prolong life and increase gamete viability can assist in the culture development of this species. The aim of this study was to evaluate the efficiency of two different cryosolutions for cryopreservation of Brazilian flounder semen in order to improve broodstock management and consequently augment the potential for its culture.Two different cryosolutions were tested: a) glycerol–saline: glycerol solution (12% or 1.65 M) along a saline-based diluent (423 mM NaCl, 9 mM KCl, 9.25 mM CaCl2.2H2O, 22.92 mM MgCl2.6H2O, 25.5 mM MgSO4.7H2O and 2.15 mM NaHCO3; pH 8.2; osmolality 900 mOsmol/kg); and b) DMSO–sucrose: DMSO solution (10% or 1.40 M) along a sucrose-based diluent (110 mM Sucrose, 100 mM KHCO3 and 10 mM Tris-Cl; pH 8.2; osmolality 335 mOsmol/kg). Cryopreservation was made without equilibration time. First, 250 μl-straws were placed 6 cm above the surface of liquid nitrogen for 10 min, then they were maintained for 5 min on the surface of liquid nitrogen (1 cm) before being plunged into liquid nitrogen. The quality of cryopreserved sperm was assessed through the percentage of sperm motility and viability, fertilization capacity, hatching and larval viability. Motility was estimated with an arbitrary scale, ranging from 0 to 5. Spermatozoa viability was determined using a LIVE/DEAD® sperm viability kit. Motility of fresh sperm (3.5±0.2) was similar to frozen/thawed sperm with DMSO-sucrose (2.5±0.3) (PN0.05). On the other hand, the motility of frozen/thawed sperm with glycerol-saline (1.3±0.4) was lower than the other two treatments (Pb0.05). No difference was found in the percentage of live spermatozoa post-thawed between DMSO–sucrose and glycerol–saline solutions (Pb0.05).However, fresh sperm had a higher percentage of live spermatozoa than post-thawed sperm with glycerol-saline (Pb0.05). Sperm motility was positively correlated with the percentage of live spermatozoa (Adjusted R2=0.61, n=13). No difference was found for fertilization and hatching rates and larvae viability among the three treatments (PN0.05). This is the first report on successful cryopreservation of Brazilian flounder sperm.This procedure should improve broodstock management techniques for this species and consequently augment the potential for its culture. pt_BR
dc.language.iso eng pt_BR
dc.rights restrict access pt_BR
dc.subject Glycerol–saline pt_BR
dc.subject DMSO–sucrose pt_BR
dc.subject Spermatozoa pt_BR
dc.subject Paralichthys orbignyanus; Reproduction pt_BR
dc.subject Reproduction pt_BR
dc.title Cryopreservation of brazilian flounder (paralichthys orbignyanus) sperm pt_BR
dc.type article pt_BR
dc.identifier.doi http://dx.doi.org/10.1016/j.aquaculture.2007.12.025 pt_BR


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