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首页> 外文期刊>Cell and tissue banking: An international journal of banking, engineering & transplantation of cells and tissues >The effect of antioxidant agents' addition and freezing method on quality parameters of frozen thawed ram semen
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The effect of antioxidant agents' addition and freezing method on quality parameters of frozen thawed ram semen

机译:抗氧化剂的添加和冷冻方法对冷冻隆型清除液体质量参数的影响

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摘要

The aim of this study was to evaluate the effect of antioxidant agents and freezing methods on the ability of ram sperm to preserve its post-thaw quality characteristics. Six Chios rams were subjected to 52 weekly semen collections. Each ram was used as semen donor for freezing experiments once every 2 weeks. Equal number of good quality spermatozoa from each ejaculate (concentration = 1 x 10(9) spermatozoa/ml, motility = 70%, motility score = 3.5) were pooled. Three equal aliquots of the pooled sample were diluted using three different fractions of a milk-based and glycerol extender (control, quercetin-enriched, alpha-tocopherol-enriched). Three freezing methods were applied (slow and fast freezing rate in a programmable freezer, vapors of liquid nitrogen) in every aliquot. Sperm aliquots were tested before freezing, immediately after thawing and after 3 h of incubation at 37 A degrees C. Sperm motility (%) was evaluated microscopically. The percentage of membrane and acrosome-intact spermatozoa (IL%) as well as the percentage of membrane-intact and acrosome-reacted spermatozoa (ARL%) were determined by eosin-nigrosin stain. Furthermore, the percentage of hypo-osmotic swelling (HOS) test-positive spermatozoa was estimated. The results revealed no beneficial effect of the antioxidant treatment on the parameters of post-thaw semen (P 0.05). However, the slow freezing rate method was more beneficial regarding motility, IL, ARL and HOS-positive spermatozoa compared to the other methods. In conclusion, the antioxidant agents used in this study failed to protect sperm against cryopreservation stress; however, the choice of the appropriate freezing method could contribute to the improvement of post-thaw ram sperm quality.
机译:本研究的目的是评估抗氧化剂和冷冻方法对ram精子保持其后解冻质量特征的影响。六条希俄斯公羊队进行了52个每周精液收集。每2周每2周使用每次RAM作为精液供体进行一次冻结实验。从每次射精(浓度& = 1×10(9)精子,运动& = 70%,运动得分和 = 3.5)的相同数量的优质精子α。使用三种不同的乳碱和甘油增量剂(对照,富含槲皮素,富含α-生育酚)稀释三等份的汇集样品的汇集样品。在每次等分试样中施加三种冷冻方法(在可编程冰箱中,液氮中的速度快速冷冻速率)。在冷冻之前测试精子等分试样,在解冻后,在37℃的37℃温育3小时后立即进行测试。微观评估精子运动(%)。通过eosin-nigrosin染色法测定膜和肌肉内完整的精子(IL%)的百分比和膜完整的精子(IL%)以及膜完整和取态反应的精子(Arl%)的百分比。此外,估计了缺血肿胀(HOS)试验阳性精子的百分比。结果表明,抗氧化剂治疗对解冻后精液的参数(P> 0.05)没有有益效果。然而,与其他方法相比,缓慢冷冻速率方法对运动,IL,ARL和HOS阳性精子更具有益。总之,本研究中使用的抗氧化剂未能保护精子免受冷冻保存应力;然而,适当的冷冻方法的选择可以有助于改善解冻后的RAM精子质量。

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