Cryopreservation of murine zygotes for use in testing culture environments

Developing one-cell mouse zygotes are more sensitive to in vitro environmental conditions than are cleavage-stage embryos. However, for convenience and reproducibility, cryopreserved two-cell zygotes are routinely used for such assays. Concern over the possibility of inducing damage by exposing one-...

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Veröffentlicht in:	Laboratory animal science (Chicago) 1997-10, Vol.47 (5), p.496-499
Hauptverfasser:	Meyer, T.K, Yurchak, M.R, Pleigo, J.F, Wincek, T.J, Dukelow, W.R, Kuehl, T.J
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Sprache:	eng
Schlagworte:	Animals BIOLOGICAL PRESERVATION Cell Survival Cells, Cultured CIGOTOS CONGELACION CONGELATION CONSERVACION BIOLOGICA CONSERVATION BIOLOGIQUE Cryopreservation - methods CULTIVO DE EMBRIONES CULTURE D'EMBRYON Culture Techniques - methods DESARROLLO EMBRIONARIO DEVELOPPEMENT EMBRYONNAIRE EMBRYO CULTURE EMBRYONIC DEVELOPMENT Ethylene Glycol - chemistry Female FREEZING MATING SYSTEMS METHODE D'ACCOUPLEMENT MICE NATURAL MATING Pregnancy RATON SISTEMAS DE APAREAMIENTO SOURIS SUPEROVULACION SUPEROVULATION ZYGOTE Zygote - cytology Zygote - physiology ZYGOTES
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container_title	Laboratory animal science (Chicago)
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creator	Meyer, T.K Yurchak, M.R Pleigo, J.F Wincek, T.J Dukelow, W.R Kuehl, T.J
description	Developing one-cell mouse zygotes are more sensitive to in vitro environmental conditions than are cleavage-stage embryos. However, for convenience and reproducibility, cryopreserved two-cell zygotes are routinely used for such assays. Concern over the possibility of inducing damage by exposing one-cell zygotes to cryoprotective agents and freeze-thaw procedures during syngamy led us to examine one-cell zygotes, with and without visible pronuclei, in an effort to minimize or avoid these effects and obtain the highest possible developmental rate. In vivo fertilized mouse zygotes were collected 21 to 43 h after administration of human chorionic gonadotropin (hCG). Suspensions of zygotes in 2M ethylene glycol were aspirated into 0.25-ml plastic insemination straws and slowly cooled at -0.5 degrees C/min to -40 degrees C before being plunged into liquid nitrogen for storage. Zygotes were thawed, rinsed, and placed in culture. Zygotes were examined initially for damage from the freeze-thaw procedure. Daily in vitro development was recorded. In this group of zygotes, no damage was apparent immediately after thawing, and a high degree of development in vitro was observed. Thus, usefulness of a cryopreservation method for one-cell murine zygotes has been confirmed
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However, for convenience and reproducibility, cryopreserved two-cell zygotes are routinely used for such assays. Concern over the possibility of inducing damage by exposing one-cell zygotes to cryoprotective agents and freeze-thaw procedures during syngamy led us to examine one-cell zygotes, with and without visible pronuclei, in an effort to minimize or avoid these effects and obtain the highest possible developmental rate. In vivo fertilized mouse zygotes were collected 21 to 43 h after administration of human chorionic gonadotropin (hCG). Suspensions of zygotes in 2M ethylene glycol were aspirated into 0.25-ml plastic insemination straws and slowly cooled at -0.5 degrees C/min to -40 degrees C before being plunged into liquid nitrogen for storage. Zygotes were thawed, rinsed, and placed in culture. Zygotes were examined initially for damage from the freeze-thaw procedure. Daily in vitro development was recorded. In this group of zygotes, no damage was apparent immediately after thawing, and a high degree of development in vitro was observed. 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However, for convenience and reproducibility, cryopreserved two-cell zygotes are routinely used for such assays. Concern over the possibility of inducing damage by exposing one-cell zygotes to cryoprotective agents and freeze-thaw procedures during syngamy led us to examine one-cell zygotes, with and without visible pronuclei, in an effort to minimize or avoid these effects and obtain the highest possible developmental rate. In vivo fertilized mouse zygotes were collected 21 to 43 h after administration of human chorionic gonadotropin (hCG). Suspensions of zygotes in 2M ethylene glycol were aspirated into 0.25-ml plastic insemination straws and slowly cooled at -0.5 degrees C/min to -40 degrees C before being plunged into liquid nitrogen for storage. Zygotes were thawed, rinsed, and placed in culture. Zygotes were examined initially for damage from the freeze-thaw procedure. Daily in vitro development was recorded. 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However, for convenience and reproducibility, cryopreserved two-cell zygotes are routinely used for such assays. Concern over the possibility of inducing damage by exposing one-cell zygotes to cryoprotective agents and freeze-thaw procedures during syngamy led us to examine one-cell zygotes, with and without visible pronuclei, in an effort to minimize or avoid these effects and obtain the highest possible developmental rate. In vivo fertilized mouse zygotes were collected 21 to 43 h after administration of human chorionic gonadotropin (hCG). Suspensions of zygotes in 2M ethylene glycol were aspirated into 0.25-ml plastic insemination straws and slowly cooled at -0.5 degrees C/min to -40 degrees C before being plunged into liquid nitrogen for storage. Zygotes were thawed, rinsed, and placed in culture. Zygotes were examined initially for damage from the freeze-thaw procedure. Daily in vitro development was recorded. In this group of zygotes, no damage was apparent immediately after thawing, and a high degree of development in vitro was observed. Thus, usefulness of a cryopreservation method for one-cell murine zygotes has been confirmed</abstract><cop>United States</cop><pmid>9355092</pmid><tpages>4</tpages></addata></record>
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subjects	Animals BIOLOGICAL PRESERVATION Cell Survival Cells, Cultured CIGOTOS CONGELACION CONGELATION CONSERVACION BIOLOGICA CONSERVATION BIOLOGIQUE Cryopreservation - methods CULTIVO DE EMBRIONES CULTURE D'EMBRYON Culture Techniques - methods DESARROLLO EMBRIONARIO DEVELOPPEMENT EMBRYONNAIRE EMBRYO CULTURE EMBRYONIC DEVELOPMENT Ethylene Glycol - chemistry Female FREEZING MATING SYSTEMS METHODE D'ACCOUPLEMENT MICE NATURAL MATING Pregnancy RATON SISTEMAS DE APAREAMIENTO SOURIS SUPEROVULACION SUPEROVULATION ZYGOTE Zygote - cytology Zygote - physiology ZYGOTES
title	Cryopreservation of murine zygotes for use in testing culture environments
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