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用于精液冷却和冷冻的驴附睾转运

Donkey Epididymal Transport for Semen Cooling and Freezing.

作者信息

Lago-Alvarez Yamilka, Podico Giorgia, Segabinazzi Lorenzo G, Cunha Lais L, Barbosa Leonardo, Arnold Carolyn E, Lima Fabio S, King Luise T, McLean Amy K, Canisso Igor F

机构信息

Department of Veterinary Clinical Medicine, College of Veterinary Medicine, University of Illinois, Urbana, IL 61801, USA.

Department of Large Animal Clinical Sciences, College of Veterinary Medicine and Biomedical Sciences, Texas A&M University, College Station, TX 77840, USA.

出版信息

Animals (Basel). 2020 Nov 25;10(12):2209. doi: 10.3390/ani10122209.

Abstract

The objectives of this study were to assess the cooling and freezing of donkey epididymal semen harvested immediately after castration (Experiment 1, = 4) or after the shipment (24 or 48 h) of epididymides attached to testicles (Experiment 2, = 14) or dissected apart (Experiment 3, = 36). In each experiment, semen was frozen immediately (Non-Centrif) in an egg yolk-based semen extender (EY) or after processing through cushion-centrifugation (Centrif) while extended in a skim milk-based extender (SC). In all three experiments, cooled, pre-freeze, and post-thaw epididymal semen was assessed for total motility (TM), progressive motility (PM), plasma membrane integrity (PMI), and high mitochondrial membrane potential (HMMP). Data were analyzed with R using mixed models and Tukey's test as posthoc. Results showed that the cooling of epididymal semen up to 24 h after harvesting did not affect motility parameters or plasma membrane integrity; furthermore, in Experiment 3, the post-thaw evaluation of both Centrif and Non-Centrif achieved similar TM and PM. Collectively, the post-thaw results revealed low motility parameters across groups; while, the PMI and HMMP did not reflect this trend, and the values remained high, suggesting that there was a lack of epididymal sperm activation with either centrifugation or extenders. In summary, freshly harvested and cooled-shipped and cooled semen had satisfactory semen parameters. Future studies need to address donkey epididymal semen fertility in mares and jennies.

摘要

本研究的目的是评估阉割后立即采集的驴附睾精液(实验1,n = 4)、或附有睾丸的附睾运输(24或48小时)后采集的精液(实验2,n = 14)、或分离后的精液(实验3,n = 36)的冷却和冷冻情况。在每个实验中,精液在基于蛋黄的精液稀释液(EY)中立即冷冻(非离心组),或在基于脱脂乳的稀释液(SC)中进行垫层离心处理(离心组)后冷冻。在所有三个实验中,对冷却、预冻和冻融后的附睾精液进行了总活力(TM)、前进活力(PM)、质膜完整性(PMI)和高线粒体膜电位(HMMP)评估。使用R软件通过混合模型和Tukey事后检验对数据进行分析。结果表明,采集后长达24小时的附睾精液冷却不影响活力参数或质膜完整性;此外,在实验3中,离心组和非离心组的冻融后评估获得了相似的TM和PM。总体而言,冻融后结果显示各实验组活力参数较低;而PMI和HMMP并未反映出这一趋势,其值仍然较高,表明离心或稀释液处理均未激活附睾精子。总之,新鲜采集、冷却运输和冷却后的精液具有令人满意的精液参数。未来的研究需要探讨驴附睾精液在母马和母驴中的生育能力。

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