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Effect of antioxidants on preservation of motility,viability and acrosomalintegrity of equine spermatozoa during storage at 5 degrees C

机译:抗氧化剂对5℃下贮藏时马精子的活力,生存力和香精的影响

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Preservation of liquid semen at 5 degreesC is an important technique in the breeding management of horses. Oxidative damage to spermatozoa during storage is a potential cause of the decline in motility and fertility during hypothermic storage of liquid semen. The objective of this study was to evaluate the use of water-soluble and lipid-soluble antioxidants to improve the maintenance of motility of equine spermatozoa at 5 degreesC during storage for 72 to 96 h. In Experiment 1, the effect of addition of catalase on the maintenance of motility, viability and acrosomal integrity was determined. Semen was collected, and these treatments were applied: catalase (0, 100 Or 200 U/mL) in nonfat, dried skim milk extender (NFDSM; with or without seminal plasma) or 10% seminal plasma + NFDSM. Motility was determined by computerized semen analysis (CASA) at 0, 24, 48 and 72 h. Viability and acrosomal integrity were determined at 72 h of storage. There was no significant treatment effect on the maintenance of sperm motility during 72 h storage, In Experiment 2, the effect of adding lipid-soluble antioxidants on maintenance of motility was evaluated. Semen was diluted to a final concentration of 25 x 10(6) sperm/mL in NFDSM containing butylated hydroxytoluene (BHT; 2.0, 1.0, or 0.5 mM), Vitamin E (4.0, 2.0, 1.0 mM), or Tempo (2.0, 1.0, or 0.5 mM). Although the addition of BHT significantly reduced (P<0.05) progressive motility during storage compared to the control, there were no positive treatment effects of either Vitamin E or Tempo on maintenance of motility. In Experiment 3, the effect of adding water-soluble antioxidants on maintenance of motility was evaluated. Semen was diluted in NFDSM containing these treatments: Trolox (2.0 mM), Tempo (1.0 mM), Vitamin C (0.45 mg/mL), BSA (3% w/v), combinations of these antioxidants, or control. Adding these water-soluble antioxidants did not significantly improve the maintenance of motility during cooled storage at 5C. In conclusion, adding the enzyme scavenger, catalase, or a variety of lipid- and water-soluble antioxidants did not significantly improve the maintenance of motility during liquid semen storage at 5 degreesC.
机译:在5°C下保存液态精液是马繁殖管理中的一项重要技术。储存过程中精子的氧化损伤可能是液体精液低温储存过程中活力和生育力下降的潜在原因。这项研究的目的是评估使用水溶性和脂溶性抗氧化剂来改善马精子在5摄氏度下储存72至96小时的运动能力。在实验1中,确定了过氧化氢酶的添加对维持运动性,生存力和顶体完整性的影响。收集精液,然后进行以下处理:过脂,干脱脂乳补充剂(NFDSM;有或没有精浆)或10%精浆+ NFDSM中的过氧化氢酶(0、100或200 U / mL)。通过计算机精液分析(CASA)在0、24、48和72小时确定运动能力。在储存72小时后测定生存力和顶体完整性。贮藏72 h期间对维持精子活力没有明显的治疗作用。在实验2中,评估了添加脂溶性抗氧化剂对维持精子活力的影响。将精液在含有丁基羟基甲苯(BHT; 2.0、1.0或0.5 mM),维生素E(4.0、2.0、1.0 mM)或Tempo(2.0, 1.0或0.5 mM)。尽管与对照相比,BHT的添加在贮藏过程中显着降低了(P <0.05)进行性运动,但维生素E或Tempo对保持运动性没有积极的治疗作用。在实验3中,评估了添加水溶性抗氧化剂对维持活力的作用。将精液在含有以下处理剂的NFDSM中稀释:Trolox(2.0 mM),Tempo(1.0 mM),维生素C(0.45 mg / mL),BSA(3%w / v),这些抗氧化剂的组合或对照。添加这些水溶性抗氧化剂并不能显着改善在5℃下冷藏时的运动能力。总之,添加酶清除剂,过氧化氢酶或各种脂类和水溶性抗氧化剂并不能显着提高液体精液在5摄氏度下储存期间的活力维持能力。

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