Application de la cryoconservation des embryons à la protection des ressources génétiques chez le lapin

Joly, Thierry; Theau-Clément, M.; Drouet-Viard, F.; Rochambeau, Hubert de; Renard, JP

doi:10.1186/1297-9686-26-s1-s267

Cited by 5 publications

(1 citation statement)

References 10 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…In vivo viability obtained from NZ vitrified embryos are in accordance with the results of Vicente and Garcfa-Xim6nez (1994) and Joly et al (1994) for vitrified and frozen embryos, respectively. These results hold promise for securing offspring from donor does.…”

Section: Experimental Animalssupporting

confidence: 83%

A sucrose-DMSO extender for freezing rabbit semen

Vicente

Viudes-de-Castro²

1996

Reprod. Nutr. Dev.

View full text Add to dashboard Cite

Summary ― The aim of this study was to define a simple extender for freezing rabbit semen from selected males used to inseminate selected does to obtain embryos for an embryo bank. Four experiments were carried out. In the first experiment, freezing extender was defined on the basis of the results of the post-thawing motility rate. Three factors and their interactions were studied: final concentration of dimethyl sulphoxide (DMSO) (1, 1.25, 1.5 and 1.75 M), egg yolk (0% of 10 v/v) and sugar (none, or 0.5 M of glucose, lactose, sucrose, or maltose). The sucrose and 1.75 DMSO improved significantly the post-thawing motility rate (sucrose 1.75 M DMSO extender: 42 ± 3%). In the second experiment, this freezing extender was used to freeze semen from three lines. The post-thawing motility and normal acrosome rates were similar among the lines when the covariates, fresh motility and normal acrosome rates, respectively, were used in the analysis (52 ± 1 and 66 ± 1 %, respectively). In the third experiment, frozen semen from the White New Zealand line (NZ) was tested by morphological normality and viability of embryos recovered. Recovery data from NZ does inseminated with fresh and frozen semen were compared. No significant differences were found in the number of normal embryos obtained per donor doe (8.9 ± 0.5) and in their survival after vitrification (52% of live foetuses at 29 days of gestation). The sucrose-DMSO extender and freezing procedure used in this work can offer satisfactory results to apply in conservation and genetic programmes.

show abstract

Section: Experimental Animalssupporting

confidence: 83%