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      Survival rates of mouse blastocyst vitrified in dimethylformamide based solutions associated with ethylene glicol or 1-2 propanediol Translated title: Sobrevivência de embriões de camundongo vitrificados em soluções com dimetilformamida associadas ao etilenoglicol ou 1-2 propanediol

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          Abstract

          The aim of this study was to determine the effect of dimethylformamide (DF) associated with ethylene glycol (EG) or 1-2 propanediol (PROH) during vitrification, on the in vitro development of mouse blastocysts. Cryoprotectant toxicity was evaluated exposing embryos into three different equilibrium solutions (ES) composed by DF, EG or PROH mixtures (10% v/v of each) in mPBS + 0.5% PVA at different interval times (1, 3 and 10min). In a second experiment, embryos were exposed to the same ES (either 1 or 3min), following for the three respectively vitrification solutions (VS) (20% v/v of each) for 30s. After 72 hours of in vitro culture, embryo hatching and expansion rates were similar for the ES1 and ES2 equilibration solutions during the time interval of 1 or 3min. However embryos exposed for 10 min to the DF equilibration solutions, had lower survival rates than EG-PROH solution (P<0.01). Furthermore, survival rates for embryos exposed to DF-PROH (ES+VS) were lower than embryos exposed to the other solutions (P<0.01). Blastocyst vitrification was performed with the three ES+VS (for 1min and 30s, respectively), using glass micropipettes (GMP). Survival rates were lower for blastocysts vitrified with DF solutions (3%-3/108 and 17.1%-19/111) (P<0.01) than with PROH+EG vitrification solutions (69%-73/105). In conclusion, DF as a cryoprotectant into vitrification solutions have deleterious effects on the in vitro developmental competence of vitrified mouse blastocysts.

          Translated abstract

          O objetivo deste estudo foi determinar o efeito da dimetilformamida (DF) associada com etileno glycol (EG) ou 1-2 propanediol (PROH) durante a vitrificação, no desenvolvimento in vitro de blastocistos murinos. A toxicidade dos crioprotetores foi avaliada ao expor os embriões as três soluções de equilíbrio (ES) compostas pelas misturas de DF, EG ou PROH (10% v/v de cada) em mPBS + 0,5% PVA, em diferentes intervalos de tempo (1, 3 e 10min). Em um segundo experimento, os embriões foram expostos as mesmas ES (durante 1 e 3min), seguido da exposição as três respectivas soluções de vitrificação (VS) (20% v/v de cada) durante 30seg. Após 72 horas de cultivo in vitro, as taxas de expansão e eclosão dos embriões expostos durante os períodos de 1 e 3min às soluções de equilíbrio ES1 e ES2 foram semelhantes. No entanto, os embriões expostos durante 10min às soluções de equilíbrio com DF apresentaram taxas de sobrevivência inferiores à solução de EG-PROH (P<0,01). Além disso, as taxas de sobrevivência dos embriões expostos à DF-PROH (ES+VS) foram menores que as dos embriões expostos as outras soluções (P<0,01). A vitrificação dos blastocistos foi realizada após a exposição dos embriões nas três ES+VS (por 1min e 30seg, respectivamente), usando micropipetas de vidro (GMP). As taxas de sobrevivência foram menores nos blastocistos vitrificados nas soluções compostas por DF (3%-3/108 e 17,1%-19/111), em relação à solução EG-PROH (69%-73/105) (P<0,01). Em conclusão, a DF adicionada como crioprotetor às soluções de vitrificação apresenta efeitos deletérios na capacidade de desenvolvimento in vitro dos blastocistos murinos vitrificados.

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          Most cited references26

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          Ice-free cryopreservation of mouse embryos at −196 °C by vitrification

          W Rall, G Fahy (1985)
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            Cryobiology: The Freezing of Biological Systems

            P. Mazur (1970)
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              Open Pulled Straw (OPS) vitrification: a new way to reduce cryoinjuries of bovine ova and embryos.

              Although cryopreservation of certain mammalian embryos is now a routine procedure, considerable differences of efficiency exist depending on stage, species and origin (in vivo or in vitro produced). Factors that are suspected to cause most of these differences are the amount of the intracellular lipid droplets and the different microtubular structure leading to chilling injury as well as the volume/surface ratio influencing the penetration of cryoprotectants. A new approach, the Open Pulled Straw (OPS) method, which renders very high cooling and warming rates (over 20,000 degrees C/min) and short contact with concentrated cryoprotective additives (less than 30 sec over -180 degrees C) offers a possibility to circumvent chilling injury and to decrease toxic and osmotic damage. In this paper we report the vitrification by the OPS method of in vitro produced bovine embryos at various stages of development. Embryos cryopreserved from Day 3 to Day 7 (Day 0 = day of fertilization) exhibited development into blastocysts at rates equivalent to those of control embryos; even those cryopreserved on Day 1 or 2 exhibited only somewhat reduced survival. Eighty-one percent of Day 8 hatched blastocysts also survived the procedure. The method was also successfully used for bovine oocytes; of 184 vitrified oocytes, 25% developed into blastocysts after fertilization and culture for 7 days. Pregnancies were achieved following transfer after vitrification at both the oocyte and blastocyst stage. The OPS vitrification offers a new way to solve basic problems of reproductive cryobiology and may have practical impact on animal biotechnology and human assisted reproduction.
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                Author and article information

                Journal
                cr
                Ciência Rural
                Cienc. Rural
                Universidade Federal de Santa Maria (Santa Maria, RS, Brazil )
                0103-8478
                1678-4596
                November 2011
                : 41
                : 11
                : 1985-1990
                Affiliations
                [01] Porto Alegre RS orgnameUniversidade Federal do Rio Grande do Sul orgdiv1Faculdade de Veterinária orgdiv2Laboratório de Embriologia e Biotecnicas da Reprodução Brasil prodriguezv@ 123456unal.edu.co
                Article
                S0103-84782011001100022 S0103-8478(11)04101122
                b2202cfb-e7e1-4b81-8103-639e459324df

                This work is licensed under a Creative Commons Attribution 4.0 International License.

                History
                : 28 April 2011
                : 11 November 2010
                Page count
                Figures: 0, Tables: 0, Equations: 0, References: 26, Pages: 6
                Product

                SciELO Brazil

                Categories
                Animal Reproduction

                glass micro pipettes,mouse,blastocyst,vitrification,dimethylformamide,camundongos,blastocistos,vitrificação,dimetilformamida,micropipetas de vidro

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