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用精子激活剂稀释的冷冻犬精液的评估

Evaluation of Chilled Dog Semen Extended With Sperm Activator.

作者信息

Martínez-Barbitta Marcelo, Rivera Salinas Claudio

机构信息

Postgraduate Program, Faculty of Veterinary Medicine, University of the Republic, Montevideo, Uruguay.

Doctorate Program, Faculty of Veterinary Medicine, University of Perugia, Perugia, Italy.

出版信息

Front Vet Sci. 2022 Feb 11;8:764750. doi: 10.3389/fvets.2021.764750. eCollection 2021.

Abstract

Within modern biotechnology, different tools and methodologies have been developed to maximize canine semen conservation protocol to optimize reproductive results. In the last decades, the survival of chilled semen has been prolonged from 2 to 3 days with the first basic diluents, to 10-14 days with the modern extenders. However, their main limitation is that sperm quality decreases during cold storage. Sperm activators (SA) have been produced to provide the molecules necessary to maximize the sperm survival and quality with the aim to enhance fertility and prolificacy. In this study, the effect of commercial extender SA (Theriosolution® Canine AI extender -Chile-) was recorded by daily evaluation of chilled semen for 14 days. In this experiment, sperm-rich ejaculate fraction was collected from six adult healthy Neapolitan Mastiff dogs. The semen evaluation started immediately after collection (d0), and after that a next generation extender was added (d0) for every 24 h from d1 (with and without SA) to d14, to determine spermatozoa progressive motility, velocity of forward progression (VFP), morphology, and integrity of the spermatic membrane. The initial sperm concentration of extended semen was 417.3 ± 170.4 x 10/mL (mean ± SEM) with 85.89 ± 4.76% of MNS (morphologically normal sperm), 84.47 ± 5.22 % live sperm, and pH of 6.2 ± 2.8. The initial VFP was 3.83 ± 0.48, but after 1 min with SA, it rises to 4.45 ± 0.45 ( < 0.001). The sperm progressive motility parameter increases significantly ( < 0.05) in experimental trial, respect to control, starting to d2 at finish (except for d7). The VFP analysis significantly increases in experimental trial ( < 0.05) during most days of the study with the exclusion of d3 and d14. To evaluate the seminal characteristics over time, the experiment was divided into T1 (d0-d5), T2 (d6-d10), and T3 (d11-d14) ( < 0.001) in evaluation of morphology and membrane functionality. The MNS reached 70% at d10 and finally 65% at d14, being considered normal and possibly fertile. With Host-s, 65% of MNS were also achieved at d14. The presence of glucose and fructose in the diluents used for refrigeration can exert very important effects given the fact that metabolic routes have been found in both sugars, providing both different and complementing effects. It can be concluded that the use of SA prior to artificial insemination improves the quality of chilled semen significantly, although it does not reverse the effects of deterioration due to cellular metabolism over time.

摘要

在现代生物技术领域,已开发出不同的工具和方法,以优化犬精液保存方案,从而实现最佳繁殖效果。在过去几十年中,冷冻精液的存活时间已从最初使用基本稀释剂时的2至3天延长至现代稀释剂下的10 - 14天。然而,其主要局限性在于精子质量在冷藏过程中会下降。已研发出精子激活剂(SA),旨在提供必要分子以最大化精子存活和质量,从而提高生育力和繁殖力。在本研究中,通过对冷藏精液进行为期14天的每日评估,记录了商业稀释剂SA(Theriosolution®犬用人工授精稀释剂 - 智利产)的效果。在该实验中,从六只成年健康那不勒斯獒犬采集富含精子的射精部分。精液评估在采集后立即开始(第0天),之后从第1天开始(添加或不添加SA),每24小时添加一次下一代稀释剂,直至第14天,以确定精子的渐进运动性、向前运动速度(VFP)、形态以及精子膜的完整性。稀释后精液的初始精子浓度为417.3 ± 170.4 x 10/mL(平均值 ± 标准误),形态正常精子(MNS)占85.89 ± 4.76%,活精子占84.47 ± 5.22%,pH值为6.2 ± 2.8。初始VFP为3.83 ± 0.48,但添加SA 1分钟后,升至4.45 ± 0.45(P < 0.001)。在实验试验中,与对照组相比,精子渐进运动性参数从第2天开始直至结束(第7天除外)显著增加(P < 0.05)。在研究的大多数日子里,除第3天和第14天外,实验试验中的VFP分析显著增加(P < 0.05)。为了评估精液特征随时间的变化,在形态和膜功能评估中将实验分为T1(第0 - 5天)、T2(第6 - 10天)和T3(第11 - 14天)(P < 0.001)。第10天时MNS达到70%,最终在第14天时为65%,可认为是正常且可能具有生育能力的。使用Host - s时,第14天也达到了65%的MNS。鉴于在用于冷藏的稀释剂中发现了葡萄糖和果糖的代谢途径,且二者具有不同但互补的作用,它们的存在可能会产生非常重要的影响。可以得出结论,人工授精前使用SA可显著提高冷藏精液的质量,尽管它无法逆转随着时间推移细胞代谢导致的精液质量下降的影响。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7a83/8874018/0dcd2006748f/fvets-08-764750-g0001.jpg

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