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Effect of Culture Condition on Hanwoo Embryonic Developments and Their Sunrival after Vitrification  

Cho, Sang-Rae (Animal Genetic Resources Station, National Institute of Animal Science, RDA)
Choi, Sun-Ho (Animal Genetic Resources Station, National Institute of Animal Science, RDA)
Choe, Chang-Yong (Animal Genetic Resources Station, National Institute of Animal Science, RDA)
Son, Jun-Kyu (Animal Genetic Resources Station, National Institute of Animal Science, RDA)
Lee, Poong-Yeon (Animal Genetic Resources Station, National Institute of Animal Science, RDA)
Ko, Yeoung-Kyu (Animal Genetic Resources Station, National Institute of Animal Science, RDA)
Kim, Hyun-Jong (Animal Genetic Resources Station, National Institute of Animal Science, RDA)
Yeon, Sung-Heum (Animal Genetic Resources Station, National Institute of Animal Science, RDA)
Son, Dong-Soo (Animal Genetic Resources Station, National Institute of Animal Science, RDA)
Publication Information
Journal of Embryo Transfer / v.25, no.3, 2010 , pp. 189-193 More about this Journal
Abstract
We investigated the cleavage rate and blastocyst yield for each culture condition to enhance tolerance of cryo-preservation of bovine IVF embryo with relatively lower cryo-tolerance compared to in vivo embryo. The cleavage rate and blastocysts yield for CR1aa, IVMD, IVD, CR1aa+10% FBS were 73.2, 69.3, 72.8, 68.5% and 44.1, 30.8, 33.3, 48.0%, respectively. The values did not differ among each treatments without serum. For embryo vitrification, In vivo and In vitro blastocysts were exposed to VS1(10% glycerin, 0.1 M glucose, 0.1 M sucrose, PEG 1%) for 5 min, and VS2 (10% glycerin, 10% EG, 0.2 M glucose, 0.2 M sucrose, PEG 2%) for 5 min and then VS3 (10% glycerin, 30% EG, 0.3 M glucose, 0.3 M sucrose, PEG 3%) for 1 min. The exposed embryos were then loaded into the 0.25 ml plastic straws and then plunged into liquid nitrogen. The straws were held for period of 1 to 2 weeks before thawing. In embryo viability, no differences in blastocyst re-expansion rates were found between in vivo and in vitro embryos. whereas expansion-BL rates was significantly higher for in vivo-derived embryos (72.7%) when compared to in vitro-derived embryos (51.4%), respectively (P<0.05). In conclusion, our results indicate that combined use of CRIaa culture medium with vitrification might enhance tolerance of cryopreservation for bovine IVF embryo production.
Keywords
bovine; embryos; in vitro; in vivo; cryopreservation;
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