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首页> 外文期刊>Theriogenology >Effect of the addition of two superoxide dismutase analogues (Tempo and Tempol) to alpaca semen extender for cryopreservation
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Effect of the addition of two superoxide dismutase analogues (Tempo and Tempol) to alpaca semen extender for cryopreservation

机译:向羊驼精液补充液中添加两种超氧化物歧化酶类似物(Tempo和Tempol)进行冷冻保存的效果

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The main objective was to study the effects, on sperm function, of the addition of two superoxide dismutase (SOD) analogues (Tempo and Tempol) to alpaca semen extender for cryopreservation. Twelve alpaca semen samples were collected using an artificial vagina and then diluted at a 1:3 ratio in an extender based on skim milk, egg yolk, and fructose. Each semen sample was divided into three equal parts to form the following groups: control, Tempo (1 mM), and Tempol (1 mM). Groups were cooled to 5 degrees C in 90 minutes (-1 degrees C in 3 minutes); when samples reached approximately 10 degrees C, SOD analogues were added to the respective groups. At 5 degrees C, ethylene glycol (final concentration, 0.1 M) was added to each group. After 30 minutes at 5 degrees C, samples were loaded in 0.25 mL plastic straws, placed in liquid nitrogen vapor for 15 minutes, and then plunged. Percentages of sperm motility, functional sperm membrane integrity, and viable sperm with intact acrosomes were evaluated before and after freeze-thaw using visual analysis, the hypo-osmotic swelling test, and the double-stain trypan blue/giemsa technique, respectively. The Terminal deoxymucleotidyl transferase dUTP Nick End Labeling assay was performed for evaluation of sperm DNA fragmentation of frozen-thawed sperm. Sperm motility was higher (P < 0.05) in the Tempol and Tempo groups than in the control group (mean, 22.1%, 19.7%, and 11.2%, respectively), with similar results for functional sperm membrane integrity. Additionally, DNA fragmentation was lower (P < 0.05) in the Tempol group (16.7%) than in the control group (38.8%). Viable sperm with intact acrosomes were not affected by the use of SOD analogues. There was a negative correlation (r = -0.58) between DNA fragmentation of alpaca sperm and sperm motility after freeze-thawing, but DNA damage was neither related to functional membrane integrity nor viable sperm with intact acrosomes. We concluded that DNA fragmentation and loss of motility during cryopreservation of alpaca sperm could be partially prevented by supplementation of the semen extender with 1 mM Tempo or Tempol
机译:主要目的是研究向羊驼精液补充液中添加两种超氧化物歧化酶(SOD)类似物(Tempo和Tempol)对精子功能的影响,以进行冷冻保存。使用人造阴道收集十二个羊驼精液样品,然后在基于脱脂牛奶,蛋黄和果糖的增量剂中以1:3的比例稀释。将每个精液样品分成三个相等的部分以形成以下组:对照,Tempo(1 mM)和Tempol(1 mM)。将各组在90分钟内冷却至5摄氏度(在3分钟内降至-1摄氏度);当样品达到约10摄氏度时,将SOD类似物添加到各个组中。在5摄氏度下,将乙二醇(最终浓度,0.1 M)添加到每组中。在5摄氏度下30分钟后,将样品装入0.25 mL塑料吸管中,置于液氮蒸气中15分钟,然后浸入。在冻融之前和之后,分别使用视觉分析,低渗溶胀试验和双重染色锥虫蓝/吉姆萨技术评估了精子运动力,功能性精子膜完整性和完整顶体的活精子百分比。进行末端脱氧核糖基转移酶dUTP缺口末端标记测定以评估冷冻融化的精子的精子DNA片段。 Tempol和Tempo组的精子运动力高于对照组(P <0.05)(分别为22.1%,19.7%和11.2%),功能性精子膜完整性的结果相似。此外,Tempol组(16.7%)的DNA片段含量低于对照组(38.8%)(P <0.05)。具有完整顶体的活精子不受SOD类似物的使用影响。羊驼精子的DNA片段与冻融后的精子活动力之间呈负相关(r = -0.58),但DNA损伤与功能性膜的完整性和完整顶体的活精子无关。我们的结论是,通过补充1 mM Tempo或Tempol精液补充剂可以部分预防冷冻羊驼精子过程中的DNA片段化和动力丧失。

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