评估精子存储温度的鸡5⁰C, 26⁰C Infuse稀释,葡萄糖5%食盐和10%

A. Asnawi, M. Maskur, A. Dradjat
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引用次数: 0

摘要

本研究的目的是比较使用NaCl、10%葡萄糖和5%葡萄糖稀释剂在26⁰C和5⁰C储存的精子的质量。收集一只公鸡的精子,将其分成6份,每2管分别用NaCl、葡萄糖5%和葡萄糖10%按1:1的比例稀释,然后每3管分别用不同的稀释剂储存在26⁰C和5⁰C。稀释后半小时、1小时观察精子活力、活力及异常情况,每2小时随访一次,直至第9小时。结果表明,在26⁰C温度下,在NaCl、10%葡萄糖和5%葡萄糖的生理稀释液中储存9小时的精子,其活力分别为50±0.0%、42±10.95,差异有统计学意义(P < 0.05)。%和34±8.94%。在5⁰C储存温度下9小时,生理NaCl、10%葡萄糖和5%葡萄糖差异显著(P0.05)。在5⁰C储存条件下,三种稀释剂的精子活力无显著差异,葡萄糖10%、葡萄糖5%和生理NaCl分别为52.57±5.15%、52.21±5.02%和48.14±8.09%。精子异常在26⁰C和5⁰C储存9小时,使用生理NaCl稀释剂,5%葡萄糖和10%葡萄糖,没有显著差异,在5%到10%之间变化。结果表明,5%葡萄糖稀释剂常温保存4 h以内的精子质量较好,NaCl稀释剂冷藏4 h以上的精子质量较高
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Evaluasi Penyimpanan Spermatozoa Ayam Pada Suhu 5⁰C, 26⁰C Dengan Pengencer Infuse NaCl, Glukosa 5% dan 10%
The purpose of this study were to compare the quality of spermatozoa stored at 26⁰C, 5⁰C using diluents of NaCl, 10% glucose and 5% glucose. The spermatozoa of a rooster was collected and divided into 6 parts, each 2 tubes diluted in a ratio of 1:1 using NaCl, Glucose5% and Glucose 10%, then each 3 tubes with different diluents were stored at 26⁰C and 5⁰C. Observations of motility, viability and abnormalities of spermatozoa were carried out half an hour, 1 hour after dilution, followed every 2 hours until the ninth hours. The results showed that spermatozoa stored for 9 hours at a temperature of 26⁰C with a physiological diluent of NaCl, 10% Glucose and 5% Glucose each were different (P, < 0.05) with motility 50 ± 0.0%, 42 ± 10.95. % and 34±8.94%, respectively. At storage temperature of 5⁰C for 9 hours, physiological NaCl, 10% glucose and 5% glucose were significantly different (P<0.05) with motility 58.00±10.95%, 46.00±8.94% and 38.00±, respectively. 10.95% in a row. The viability of spermatozoa at 26⁰C storage with 5% glucose diluent was better than 10% glucose and physiological NaCl (P<0.05), 58.93±1.27%, 42.93±1.48% and 33.43±1.27% , while the physiological NaCl diluent and 10% glucose were not significantly different (P>0.05). At 5⁰C storage the viability of spermatozoa in the three diluents was not significantly different, with values of Glucose 10%, Glucose 5% and physiological NaCl 52.57±5.15%, 52.21±5.02% and 48.14±8.09%, respectively. Spermatozoa abnormalities at storage temperature 26⁰C and 5⁰C for 9 hours using physiological NaCl diluent, 5% glucose and 10% glucose, were not significantly different and varied between 5 to 10%. Finally, it can be concluded that at room temperature storage less than 4 hours the quality of spermatozoa was better with 5% glucose diluent, while for cold storage beyond 4 hours the quality of spermatozoa with NaCl diluent was higher
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