光刺激对冻融公牛精子生殖潜能影响的评价。

IF 0.8 4区 农林科学 Q3 VETERINARY SCIENCES Polish journal of veterinary sciences Pub Date : 2022-06-01 DOI:10.24425/pjvs.2022.141809
A D Ömür
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引用次数: 1

摘要

本研究的目的是利用多波长LED(发光二极管)确定光刺激对牛精子细胞的时间依赖性效果。对精子学参数进行活力、顶体结构和活力的评价。此外,光刺激对体外获能的冻融精子细胞的影响从线粒体膜电位的变化方面进行了评估。这项研究包括两个独立的实验,总共使用了32个来自不同公牛的精子样本。所有的精子样本都是通过人工阴道从荷斯坦公牛身上获得的。在0.25 ml吸管中,将精液稀释至每ml 92 × 106个精子的最终浓度。使用常规方法冷冻精细胞。吸管在37°C水浴中保存20秒,并在磷酸缓冲盐水(PBS)中稀释1:4,以消除甘油的潜在有害作用,甘油是公牛精子冷冻介质中主要的渗透性冷冻保护剂。这种稀释也有助于评估精子质量参数。在第一个试验中,15-10-15处理与对照没有差异,而其他处理如10-10-10、5-5-5和3-1-3处理在24h时的活精子百分比显著高于对照。顶体完整性的结果与精子活力评估中观察到的结果非常相似。实际上,虽然由15-10-15组成的治疗没有积极效果,但较短的治疗产生了更积极的效果。2-1-2和1-1-1的顶体完整精子百分比显著高于对照。在光刺激后0、2、4和24h,除15-10-15外,所有处理的线粒体膜电位均有显著差异。高线粒体膜电位的精子百分比在10-10-10、5-5-5和3-1-3处理中增加最多。总运动力和进行性运动力方面,10-10-10是最佳方案,5-5-5和3-1-3处理也有积极作用。然而,在2h和4h时,15-10-15似乎对进行性运动有刺激作用,但随后下降,与24h时的对照组相比没有显着差异。在第二个实验中,不是在解冻后立即进行,而是在室温下保存24小时后,我们观察到光刺激组与对照组在活力、顶体完整性和总/渐进运动性方面没有统计学差异。这表明,当解冻后的精子没有立即受到刺激时,光刺激就不能发挥有益的作用。结果表明,以10-10-10、5-5-5、3-1-3和2-1-2的模式进行光刺激,在较小程度上增加了冻解冻公牛精子的恢复力。
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Evaluation of the effects of photostimulation on freeze-thawed bull sperm cells in terms of reproductive potential.
The aim of this study was to determine the time-dependent effectiveness of photo-stimulation against bovine sperm cells using a multi-wavelength LED (Light Emitting Diode). Spermatological parameters were evaluated for viability, acrosome structure and motility. In addition, the effect of photo-stimulation on frozen-thawed sperm cells subjected to in vitro capacitation was evaluated in terms of changes in mitochondrial membrane potential. The study consisted of two separate experiments and a total of 32 sperm samples obtained from separate bulls were used. All sperm samples were obtained from Holstein bulls using an artificial vagina. Semen was diluted to a final concentration of 92 x 106 spermatozoa per ml in 0.25 ml straws. The sperm cells were frozen using the conventional method. Straws were kept in a 37°C water bath for 20 seconds and diluted 1:4 in phosphate buffered saline (PBS) to eliminate the potentially deleterious effect of glycerol, the main permeable cryoprotectant in the freezing medium for bull sperm. This dilution also helped in the evaluation of sperm quality parameters. In the first experiment, whereas the 15-10-15 showed no differences with the control, other treatments such as 10-10-10, 5-5-5, and 3-1-3 exhibited significantly higher percentages of viable spermatozoa at 24h. The results obtained for acrosome integrity were pretty much similar to those observed in the sperm viability assessment. In effect, while the treatment consisting of 15-10-15 had no positive effects, shorter treatments exerted a much more positive effect. The percentages of acrosome-intact spermatozoa in 2-1-2 and 1-1-1 were significantly higher than those obtained in the control. The significant differences in mitochondrial membrane potential were observed at 0, 2, 4 and 24h post-photo-stimulation in all treatments, except 15-10-15. The highest increase in the percentage of spermatozoa exhibiting high mitochondrial membrane potential was found in 10-10-10, 5-5-5 and 3-1-3 treatments. With regard to total and progressive motility, whereas 10-10-10 was the best regime, 5-5-5 and 3-1-3 treatments also had a positive effect. However, 15-10-15 appeared to have a stimulating effect upon progressive motility at 2h and 4h but later declined and showed no significant differences with regard to the control at 24h. In the second experiment, not immediately after thawing but after having been kept at room temperature for up to 24h, it was observed that there was no statistical difference in terms of viability, acrosome integrity and total/progressive motility between photostimulation and the control group. This indicates that photo- stimulation is less able to exert a beneficial effect when post-thawed sperm are not immediately stimulated. As a result it was determined that photo-stimulation at a pattern of 10-10-10, 5-5-5, 3-1-3 and, to a lesser extent 2-1-2, increases the resilience of frozen-thawed bull sperm when applied upon thawing.
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来源期刊
Polish journal of veterinary sciences
Polish journal of veterinary sciences 农林科学-兽医学
CiteScore
1.40
自引率
0.00%
发文量
60
审稿时长
12-24 weeks
期刊介绍: Polish Journal of Veterinary Sciences accepts short communications, original papers and review articles from the field of, widely understood, veterinary sciences - basic, clinical, environmental, animal-origin food hygiene, feed hygiene, etc.
期刊最新文献
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