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Improvement in cryosurvival of buffalo bull (Bubalus bubalis) sperm by altering freezing rate within critical temperature range

机译:通过改变临界温度范围内的冷冻速率来改善水牛公牛的冷冻存活率

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摘要

Objective:To optimize the cryopreservation of buffalo bull semen by altering freezing rates within critical temperature range (4℃ to -60℃). Methods: A total of 20 ejaculates each from 5 Murrah buffalo bulls were cryopreserved using programmable biofreezer in 2 phases. In the 1st phase, 9 freezing rates were applied at -2, -5, -10, -20, -30, -40, -50, -60 or -4℃/min (control) from 4℃ to -15℃; at -40℃/min from -15℃ to -60℃. In the 2nd phase, a fixed freezing rate was applied at -30℃/min from 4℃ to -15℃. Six freezing rates were applied at -10, -20, -30, -40 (control), -50 or -60℃/min from -15℃ to -60℃. The freezing from -60℃ to -140℃ were fixed at -50℃/min in both the phases. Post thaw semen quality was assessed in terms of motility, viability, membrane integrity (hypo-osmotic swelling test), sperm abnormalities, and active mitochondria. Data were arc sine transformed and analyzed through one-way analysis of variance using SPSS software. Results: In the 1st phase, percent individual motility, progressive motility and viability were similar among various protocols. Percent hypo-osmotic swelling reactive sperm was higher with freezing at -30℃/min. In the 2nd phase, percent individual motility, viability and hypo-osmotic swelling reactive sperm was higher with freezing at -50℃/min. Sperm head abnormalities were lower at -30℃/min in the 1st phase, but were similar among the protocols of the 2nd phase. Percent active mitochondria were higher at -30℃/min in the 1st phase and at -50℃/min in the 2nd phase.Conclusions:The optimum post thaw semen quality of buffalo bull could be obtained by applying freezing rate at -30℃/min (4℃ to -15℃) and at -50℃/min (-15℃ to -140℃), followed by plunging of straws in into liquid nitrogen for storage.
机译:目的:通过改变临界温度范围(4℃至-60℃)内的冷冻速度来优化水牛的精液冷冻保存。方法:使用可编程生物冷冻机分两期对5头Murrah水牛公牛的20粒精液进行冷冻保存。在第1阶段,以2,-5,-10,-20,-30,-40,-50,-60或-4℃/ min(对照)的9个冷冻速率从4℃到-15℃ ;从-15℃到-60℃以-40℃/ min的速度运转。在第二阶段中,以-30℃/ min的速率从4℃到-15℃采用固定的冷冻速率。从-15℃到-60℃,以-10,-20,-30,-40(对照),-50或-60℃/ min的速度进行六次冷冻。在两个阶段中,从-60℃至-140℃的冻结均固定为-50℃/ min。根据运动能力,生存力,膜完整性(低渗溶胀试验),精子异常和活跃的线粒体评估了解冻后精液的质量。使用SPSS软件对数据进行反正弦变换并通过单向方差分析进行分析。结果:在第一阶段,各种方案之间的个体运动百分比,进行性运动和生存力相似。在-30℃/ min冻结时,低渗透性反应性精子的百分比更高。在第二阶段,以-50℃/ min的速度冷冻时,个体运动力,生存力和低渗溶胀反应性精子的百分比更高。在第一阶段,精子头异常在-30℃/ min时较低,但在第二阶段中相似。第一阶段的线粒体活性百分比在-30℃/ min时较高,而在第二阶段则为-50℃/ min。结论:采用-30℃/ min的冷冻速度可获得最佳的解冻后水牛精液质量。分钟(4℃至-15℃)和-50℃/ min(-15℃至-140℃),然后将吸管插入液氮中进行存储。

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  • 来源
    《亚太生殖杂志(英文版)》 |2018年第2期|72-78|共7页
  • 作者单位

    Department of Veterinary Gynaecology and Obstetrics, Guru Angad Dev Veterinary and Animal Sciences University, Ludhiana 141004, Punjab India;

    Department of Veterinary Gynaecology and Obstetrics, Guru Angad Dev Veterinary and Animal Sciences University, Ludhiana 141004, Punjab India;

    Department of Buffalo Physiology and Reproduction, Central Institute for Research on Buffalo, Hisar 125001, Haryana, India;

    Department of Veterinary Gynaecology and Obstetrics, Guru Angad Dev Veterinary and Animal Sciences University, Ludhiana 141004, Punjab India;

    Department of Veterinary Gynaecology and Obstetrics, Guru Angad Dev Veterinary and Animal Sciences University, Ludhiana 141004, Punjab India;

    Department of Veterinary Gynaecology and Obstetrics, Guru Angad Dev Veterinary and Animal Sciences University, Ludhiana 141004, Punjab India;

    Livestock Farms Complex, Guru Angad Dev Veterinary and Animal Sciences University, Ludhiana 141004, Punjab India;

    Department of Veterinary Gynaecology and Obstetrics, Guru Angad Dev Veterinary and Animal Sciences University, Ludhiana 141004, Punjab India;

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