RESUMO
The aim of this work was to study of the effect of the amino acids (AA) taurine (T) and hypotaurine (H) and of different calcium ionophore concentrations on the ability of capacitated frozen-thawed dog sperm to undergo the acrosome reaction (AR). Fifteen ejaculates grouped into five pools were used. Sperm was frozen at a concentration of 80x10(6)sperm cells/mL in the Uppsala Equex extender (UE) supplemented with 25, 50 and 75mM of either AA. The UE extender without T or H was used as control. After thawing, sperm was capacitated with Canine Capacitation Medium for 20min. Sperm was then challenged with calcium ionophore A23178 at 0, 2.5 and 10microM concentration and evaluated for integrity of plasma and acrosome membranes after 5, 15 and 30min of incubation, utilizing PI/Fitc-PNA fluorescent staining and flow cytometry. Sperm cryopreserved in UE supplemented with 50mM T (UE 50T) had higher AR rates than sperm cryopreserved with UE 75T, UE 25H and UE 50H, but AR rates were similar to semen frozen with the control extender. Challenges with 2.5 and 10microM/L of calcium ionophore increased AR in frozen-thawed sperm incubated for 5, 15 and 30min. The combination of calcium ionophore concentration and incubation time resulting in the highest AR rate was 10microM and 15min.
Assuntos
Acrossomo/metabolismo , Acrossomo/fisiologia , Ionóforos , Preservação do Sêmen/métodos , Taurina/análogos & derivados , Animais , Criopreservação/veterinária , Crioprotetores/farmacologia , Cães , MasculinoRESUMO
The working hypothesis of the present study was that supplementation of the Uppsala Equex II (UE) extender with the amino acid (AA), taurine (T) and hypotaurine (H) would improve dog sperm post-thaw quality, as previously seen for ram and bull semen, respectively. Five pools from 15 ejaculates of 15 dogs were used. Each AA was added to the UE extender at a concentration of 25, 50 and 7 5mM. Amino acid-free extender was used as a control. The following post-thaw parameters were evaluated: sperm motility by light microscopy and by CASA evaluation, longevity, viability (eosin-nigrosin staining), and flow cytometry (FC) was used to assess acrosome integrity and mitochondrial activity after PI/Fitc-PSA and PI-Rhodamine staining, respectively. Post-thaw sperm motility and velocity did not differ among extenders. Amplitude of lateral head displacement was lower for sperm frozen in the 25 mM H-supplemented extender. Semen frozen in the extender with 50 mM of T resulted in higher number of live sperm with damaged acrosomes after thawing. Higher numbers of live sperm with minimal mitochondrial activity were obtained for samples frozen with 25 and 50 mM T-supplemented extenders. Semen frozen in the control and 50 mM T-supplemented extenders had the highest number of live (eosin-nigrosin stain negative) sperm immediately post-thawing. We concluded that supplementation of the Uppsala extender with T or H did not improve sperm post-thaw mitochondrial activity or semen motility and viability.