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Cryopreservation of in vitro produced bovine embryos: effects of lipid segregation and post-thaw laser assisted hatching

机译:冷冻保存体外产生的牛胚胎:脂质分离和融化后激光辅助孵化的影响

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The objective was to determine if lipid segregation, with or without post-thaw laser assisted hatching (LAH) of in vitro produced (IVP) bovine embryos, would enhance in vitro survivability and development 24 h post-thaw. On Day 6 of culture (Day 0 = IVF), in vitro produced bovine embryos were divided into three developmental stages: 32-cell (n = 78), compact morula (CM n = 223), and blastocyst (n =56). Embryos within each stage were allocated to the following treatments prior to cryopreservation in 1.5M ethylene glycol: no treatment (Control), 7.5 mu g/mL Cytochalasin B for 20 min (CB), or CB with centrifugation (16,000 X g) for 20 min (CBCF). All CB treatments were extended to include embryo freezing. Immediately post-thaw, one-half of the CBCF and Control groups were subjected to zona pellucida drilling (LAH), using the XY Clone (R) system, creating groups CBCFLAH and LAH, respectively. All thawed embryos were cultured for 24 h and evaluated. No treatment differences were observed for either post-thaw survival or 24 h development. Within the CM stage, CBCFLAH and LAH exhibited a greater number of both total and live cells than Control (total: 69.4, 69.3, 53.0, live: 56.4, 54.7, 39.3 respectively; P < 0.05). In conclusion, LAH post-thaw alone or in combination with CBCF improved embryo viability following cryopreservation
机译:目的是确定在有或没有体外产生的(IVP)牛胚胎的融化后激光辅助孵化(LAH)的情况下,脂质的分离是否会提高融化后24 h的体外存活率和发育。在培养的第6天(第0天= IVF),将体外产生的牛胚胎分为三个发育阶段:32细胞(n = 78),紧密桑(CM n = 223)和胚泡(n = 56)。在冷冻保存于1.5M乙二醇中之前,将每个阶段的胚胎分配给以下处理:不处理(对照),7.5μg / mL细胞松弛素B 20分钟(CB)或离心CB(16,000 X g)20分钟(CBCF)。所有的CB治疗都扩展到包括胚胎冷冻。解冻后,立即使用XY Clone(R)系统对CBCF和对照组的一半进行透明带钻(LAH),分别创建CBCFLAH和LAH组。将所有解冻的胚胎培养24小时并评估。解冻后存活或24小时发育均未观察到治疗差异。在CM阶段,CBCFLAH和LAH的总细胞和活细胞数量均比对照多(总数:分别为69.4、69.3、53.0,活:56.4、54.7、39.3; P <0.05)。总之,LAH单独或与CBCF融化后可提高冷冻保存后的胚胎活力

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