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Cryopreservation of canine ovarian cortex using DMSO or 1,3-propanediol

机译:使用DMSO或1,3-丙二醇冷冻保存犬卵巢皮质

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Cryopreservation of ovarian cortex is potentially an important tool for the conservation of endangered species. It will allow preserving the large pool of primordial and primary follicles to retrieve fertilizable oocytes in the future. The aim of this study was to evaluate the effects of slow freezing on the morphology and viability of canine follicles after thawing using DMSO or 1,3-propanediol (PROH) as cryoprotectants. Slices of canine ovarian tissue were equilibrated for 20 minutes at 20 degrees C in minimum essential medium containing either cryoprotectants at 1.5 M, and then frozen by a standardized protocol. Morphology of follicles after thawing was analyzed by means of histology and transmission electron microscopy, and viability was assessed using Trypan blue and fluorescent probes. The exposure of dog ovarian tissue to both cryoprotectants before freezing had no effect on follicular morphology and viability. Also after freezing, follicles remained histologically normal, but transmission electron microscopy revealed damage of ultra structure in follicles, which were exposed to PROH. Postthaw viability was significantly reduced with 65.7% of the follicles remaining alive in DMSO and 48.7% in PROH. In conclusion, this study demonstrated the survival of canine oocytes within ovarian cortex cryopreserved by slow freezing using 1.5-M DMSO. (C) 2016 Elsevier Inc. All rights reserved.
机译:卵巢皮质的冷冻保存可能是保护濒危物种的重要工具。将来,它将保留大量的原始卵泡和初级卵泡以回收可受精的卵母细胞。这项研究的目的是评估使用DMSO或1,3-丙二醇(PROH)作为冷冻保护剂解冻后缓慢冷冻对犬卵泡形态和活力的影响。将犬卵巢组织切片在含有1.5M冷冻保护剂的最低基本培养基中于20°C平衡20分钟,然后通过标准化方案冷冻。通过组织学和透射电子显微镜分析融化后的卵泡形态,并使用锥虫蓝和荧光探针评估生存力。冷冻前将狗卵巢组织暴露于两种冷冻保护剂中对卵泡的形态和生存能力没有影响。同样在冷冻后,卵泡在组织学上仍保持正常,但是透射电镜显示暴露于PROH的卵泡的超微结构受损。解冻后的存活率显着降低,DMSO中有65.7%的卵泡存活,而PROH中有48.7%。总之,这项研究证明了使用1.5 M DMSO缓慢冷冻后冷冻保存的卵巢皮质中的犬卵母细胞的存活率。 (C)2016 Elsevier Inc.保留所有权利。

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