Cryoprotective effect of different glycerol concentrations on domestic cat spermatozoa

Villaverde, Ana Izabel Silva Balbin; Fioratti, Eduardo Gorzoni; Penitenti, Marcimara; Ikoma, Maura Rosane Valério; Tsunemi, Miriam Harumi; Papa, Frederico Ozanam; Lopes, Maria Denise

doi:10.1016/j.theriogenology.2013.06.010

Cited by 36 publications

(32 citation statements)

References 34 publications

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“…The subsequent fast cooling step from 10 or even 15 to 4°C, which was in our case already part of the freezing process over liquid nitrogen, was well tolerated by cat epididymal sperm. In the samples only cooled to 15°C, the velocity of progressive sperm after cryopreservation was the only parameter which was immedi- AE 12 (Villaverde et al 2013) ately after thawing significantly reduced in relation to samples which had been further cooled to 10°C (and in relation to initial values). On the contrary, the linearity of progressive sperm after thawing was higher after cooling to only 15 than to 10°C.…”

Section: Discussionmentioning

confidence: 88%

“…Cooling rates between À0.5 and À0.1 K/min were probably used in most studies even if exact rates and final temperatures achieved during cooling are not always reported in detail. However, (Villaverde et al 2013) used a faster cooling rate of À3.4 K/min and (Zambelli et al 2002) was successful with a cooling rate of À12 K/min in the presence of glycerol followed by a subsequent holding step at 4°C (Table 3). This holding step can be attributed to sperm equilibration with glycerol, to sperm adaptation to 4°C or both.…”

Section: Discussionmentioning

confidence: 99%

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Successful Cryopreservation of Domestic Cat (Felis catus) Epididymal Sperm after Slow Equilibration to 15 or 10°C

Klaus

Eder

Franz

et al. 2016

Reprod Domestic Animals

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To support conservation strategies in wild species, simple but highly reproducible procedures of sperm cryopreservation are required for an application under field conditions. We used epididymal sperm of the domestic cat to optimize a sperm freezing procedure for felid species, particularly questioning the demand for sperm cooling to 4°C. We equilibrated sperm during slow cooling to only 15 or 10°C in a Tes-Tris-fructose extender with final concentrations of 4.7% (v/v) glycerol and 10% (v/v) of the water-soluble fraction of hen's egg yolk (low-density lipoproteins). Subsequently, sperm were frozen over liquid nitrogen. Total and progressive motility (mean ± SD) after thawing was 60.7 ± 8.6% and 53.9 ± 9.6% in samples cooled to 15°C or 61.6 ± 9.5% and 55.3 ± 9.9% in samples cooled to 10°C. Therefore, a one-step addition of glycerol to sperm at room temperature together with the freezing extender, the use of cryovials (loaded with diluted sperm aliquots of 300 μl), an equilibration period of 40 min comprising slow cooling to 15°C at a rate of approximately -0.14 K/min before rapid freezing over liquid nitrogen, yielded satisfying results. Cooling, freezing and thawing rates were exactly characterized as a prerequisite for further optimization and to provide a repeatable protocol to other practitioners.

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Section: Discussionmentioning

confidence: 88%

Section: Discussionmentioning

confidence: 99%

Successful Cryopreservation of Domestic Cat (Felis catus) Epididymal Sperm after Slow Equilibration to 15 or 10°C

Klaus

Eder

Franz

et al. 2016

Reprod Domestic Animals

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“…Iodixanol can be postulated to be a cryoprotectant similar to sugar, ethylene glycol and glycerol. Glycerol is widely accepted as having a lower freezing point in the intracellular process of spermatozoa in livestock (Villaverde et al 2013). In the present study, it was found that a low concentration of 2.50% iodixanol in the extender (together with glycerol in the TEY dilution) had a less toxic effect on the motility of frozen sperm; similar results have been previously reported (Saragusty et al 2009;Cirit et al 2013).…”

Section: Discussionmentioning

confidence: 99%

Effects of supplementation of iodixanol to semen extender on quality and fertilization ability of frozen–thawed Thai native bull sperm

Chuawongboon

Sirisathien

Pongpeng

et al. 2017

Animal Science Journal

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This study investigates the effects of iodixanol supplementation in varied concentrations to Tris egg yolk (TEY) extender on the quality and fertilization ability of frozen-thawed sperm of Thai native bulls. Each ejaculate was divided into four different groups, as follows: sperm were treated with TEY extender (control group) and TEY extender supplemented with three different concentrations of iodixanol (1.25%, 2.50% and 5.00%). Semen straws were frozen in liquid nitrogen vapor. After thawing, sperm motility characteristics, viability, plasma membrane integrity and acrosome integrity were determined. Also, frozen-thawed spermatozoa from all groups were used for in vitro fertilization and artificial insemination (AI) in natural estrus Thai native cows. The results showed that the post-thaw quality of the 2.50% iodixanol group was superior to the other iodixanol groups (P < 0.05). However, iodixanol had no beneficial effect on post-thaw sperm in vitro fertilization ability and pregnancy rate after AI (P > 0.05). It can be concluded that the supplementation of 2.50% iodixanol extender significantly improves the progressive motility, viability, plasma membrane integrity and acrosome integrity of cryopreserved semen from Thai native bulls, but it has no beneficial effect on in vitro fertilization ability and pregnancy rate after AI.

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“…Assim, recomenda-se para o gato, a adição do glicerol a 4ºC, a fim de minimizar os efeitos tóxicos do crioprotetor, em concentrações inferiores a 8%, sendo que o emprego deste a 5% confere melhor efeito crioprotetor à célula espermática (Deco- Souza et al, 2013;VillaVerde et al, 2013).…”

Section: Criopreservação Dos Espermatozoides Epididimáriosunclassified

“…Quanto à descongelação, várias são as temperaturas (37ºC, 38ºC, 42ºC, 65ºC, 70ºC) e tempos (6 a 30 segundos) propostos (Axner et al, 2004;Chatdarong et al, 2007;Cocchia et al, 2010;Vick et al, 2012;VillaVerde et al, 2013;Vizuete et al, 2014;Buranaamnuay, 2015;Thuwanut et al, 2015;Klaus et al, 2016;Kunkitti et al, 2016). A escolha do protocolo de descongelação dependerá da curva de congelação estabelecida, sendo assim, espermatozoides submetidos à refrigeração lenta são submetidos a tempo maior de descongelação (Buranaamnuay, 2017).…”

Section: Criopreservação Dos Espermatozoides Epididimáriosunclassified

Recuperação e conservação de espermatozoides epididimários: Perspectivas e aplicações na espécie felina doméstica

et al. 2019

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Recuperação e conservação de espermatozoides epididimários: Perspectivas e aplicações na espécie felina doméstica[Recovery and conservation of epididymal sperm: Prospects and applications in the domestic feline species] Resumo A recuperação e criopreservação dos espermatozoides epidídimários é uma ferramenta promissora no resgate e/ou prevenção da perda de material genético de machos valiosos ou estimados, ou mesmo, de animais em risco de extinção. A conservação destes espermatozoides na espécie felina doméstica ainda apresenta resultados conflitantes, dificultando a aplicação da biotécnica na área comercial, para animais de padrão racial desejado. Contudo, inúmeras pesquisas investigam as peculiaridades fisiológicas dos espermatozoides felinos, com o intuído de desenvolver protocolos e meios de criopreservação promissores. Assim, alguns trabalhos já reportaram sucesso na congelação dos espermatozoides epididimários de gatos, bem como, no emprego destas células em técnicas de reprodução assistida (inseminação artificial e fecundação in vitro). Portanto, o presente artigo tem como finalidade explanar os principais avanços na área da recuperação e conservação dos espermatozoides epididimários para os gatos domésticos e, enfatizar as perspectivas futuras destes trabalhos na conservação do germoplasma felino.Palavras-chave: espermatozoide felino; epidídimo; recuperação de espermatozoides; criopreservação. AbstractThe recovery and cryopreservation of epididymal sperm is a promising tool in the rescue and prevention of loss of genetic material from valuable and/or estimated males, or even animals at risk of extinction. The conservation of these gametes in the domestic feline species still presents conflicting results, hindering the application of this biotechnology in the commercial area for animals of the desired racial pattern. However, numerous studies investigate the physiological peculiarities of feline sperm with the objective of developing promising cryopreservation protocols and means. Thus, some studies have reported success in the freezing of epididymal sperm, as well as in the use of these cells in assisted reproduction techniques (artificial insemination and in vitro fertilization). Therefore, this article aims to explain the main advances in the area of recovery and conservation of epididymal sperm for domestic cats and to emphasize the future prospects of this work in the conservation of feline germplasm.

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Cryoprotective effect of different glycerol concentrations on domestic cat spermatozoa

Cited by 36 publications

References 34 publications

Successful Cryopreservation of Domestic Cat (Felis catus) Epididymal Sperm after Slow Equilibration to 15 or 10°C

Successful Cryopreservation of Domestic Cat (Felis catus) Epididymal Sperm after Slow Equilibration to 15 or 10°C

Effects of supplementation of iodixanol to semen extender on quality and fertilization ability of frozen–thawed Thai native bull sperm

Recuperação e conservação de espermatozoides epididimários: Perspectivas e aplicações na espécie felina doméstica

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