首页> 外文期刊>Cryobiology: International Journal of Low Temperature Biology and Medicine >Cryopreservation of rainbow trout (Oncorhynchus mykiss) blastomeres:Influence of embryo stage on postthaw survival rate
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Cryopreservation of rainbow trout (Oncorhynchus mykiss) blastomeres:Influence of embryo stage on postthaw survival rate

机译:虹鳟卵裂球冷冻保存:胚胎期对解冻后存活率的影响

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The cryopreservation of isolated fish blastomeres is likely to provide a valid alternative to embryo cryopreservation, the results of which are still discouraging. A repeatable technique for the cryopreservation of rainbow trout blastomeres has been established and the effect of embryonic developmental stage on freezing tolerance evaluated. Embryos at Ballard 6A, 6B, and 6C stages were dechorionated and left to dissociate in a Ca2+- and Mg2+-free medium. Cryoprotection was provided by step-wise addition of 1.4 M 1,2-propanediol. Cells were loaded into the middle of 250-mu l straws and slowly frozen to -80 degrees C before being plunged into LN2. A low thawing rate was adopted, followed by step-wise removal of the cryoprotectant. Morphological evaluation was by microscopy and video recording. Metabolic activity and survival rate were determined by FDA and PI staining, by recovery of the ability to reassociate after 24 h culture in Leibovitz L15 + 2% Ultroser, and by measuring DNA synthesis in 6B cells by the method of BrdU incorporation. Survival rates were 53 +/- 9.3, 88 +/- 1.7, and 95 +/- 0.5% for stage 6A, 6B, and 6C cells, respectively. While 6A cells reassociated into clumps of cells, 6B and 6C cells formed holoblastic morulas in 24 h; proliferation of 6B cells was comparable to fresh control cells. The relationship between freezing tolerance and the physiological events occurring during early embryonic development is discussed in light of these results and conclusions are drawn that envisage the transfer of frozen-thawed blastomeres into recipient embryos.
机译:分离的鱼卵裂球的冷冻保存可能为胚胎冷冻保存提供有效的替代方法,其结果仍然令人沮丧。建立了虹鳟卵裂球冷冻保存的可重复技术,并评估了胚胎发育阶段对耐寒性的影响。将Ballard 6A,6B和6C阶段的胚胎去绒毛,并使其在不含Ca2 +和Mg2 +的培养基中解离。通过逐步加入1.4 M 1,2-丙二醇来提供低温保护。将细胞装入250 ul吸管的中间,并缓慢冷冻至-80摄氏度,然后再放入LN2中。采用低解冻速率,然后逐步除去冷冻保护剂。通过显微镜和视频记录进行形态学评估。通过FDA和PI染色,通过在Leibovitz L15 + 2%Ultroser中培养24小时后恢复缔合的能力以及通过采用BrdU掺入法测量6B细胞中的DNA合成来确定代谢活性和存活率。 6A,6B和6C期细胞的存活率分别为53 +/- 9.3、88 +/- 1.7和95 +/- 0.5%。当6A细胞重新结合成团块时,6B和6C细胞在24小时内形成了绒毛状桑。 6B细胞的增殖与新鲜对照细胞相当。根据这些结果,讨论了冷冻耐受性与早期胚胎发育过程中发生的生理事件之间的关系,并得出了将冷冻融化的卵裂球转移到受体胚胎中的结论。

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