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淡水鱼(欧亚鲈,河鲈)和海水鱼(欧洲鳗鲡,鳗鲡)精子玻璃化冷冻方案的开发。

Development of sperm vitrification protocols for freshwater fish (Eurasian perch, Perca fluviatilis) and marine fish (European eel, Anguilla anguilla).

作者信息

Kása Eszter, Bernáth Gergely, Kollár Tímea, Żarski Daniel, Lujić Jelena, Marinović Zoran, Bokor Zoltán, Hegyi Árpád, Urbányi Béla, Vílchez M Carmen, Morini Marina, Peñaranda David S, Pérez Luz, Asturiano Juan F, Horváth Ákos

机构信息

Department of Aquaculture, Szent István University, Páter Károly u. 1., H-2100 Gödöllő, Hungary.

Department of Aquaculture, Szent István University, Páter Károly u. 1., H-2100 Gödöllő, Hungary.

出版信息

Gen Comp Endocrinol. 2017 May 1;245:102-107. doi: 10.1016/j.ygcen.2016.05.010. Epub 2016 May 9.

DOI:10.1016/j.ygcen.2016.05.010
PMID:27174751
Abstract

Vitrification was successfully applied to the sperm of two fish species, the freshwater Eurasian perch (Perca fluviatilis) and marine European eel (Anguilla anguilla). Sperm was collected, diluted in species-specific non-activating media and cryoprotectants and vitrified by plunging directly into liquid nitrogen without pre-cooling in its vapor. Progressive motility of fresh and vitrified-thawed sperm was evaluated with computer-assisted sperm analysis (CASA). Additional sperm quality parameters such as sperm head morphometry parameters (in case of European eel) and fertilizing capacity (in case of Eurasian perch) were carried out to test the effectiveness of vitrification. The vitrification method for Eurasian perch sperm resulting the highest post-thaw motility (14±1.6%) was as follows: 1:5 dilution ratio, Tanaka extender, 30% cryoprotectant (15% methanol+15% propylene-glycol), cooling device: Cryotop, 2μl droplets, and for European eel sperm: dilution ratio 1:1, with 40% cryoprotectant (20% MeOH and 20% PG), and 10% FBS, cooling device: Cryotop, with 2μl of sperm suspension. Viable embryos were produced by fertilization with vitrified Eurasian perch sperm (neurulation: 2.54±1.67%). According to the ASMA analysis, no significant decrease in head area and perimeter of vitrified European eel spermatozoa were found when compared to fresh spermatozoa.

摘要

玻璃化冷冻技术已成功应用于两种鱼类的精子,即淡水欧洲鲈鱼(河鲈)和海洋欧洲鳗鲡。收集精子,在特定物种的非激活培养基和冷冻保护剂中稀释,然后直接投入液氮中进行玻璃化冷冻,无需在液氮蒸汽中预冷。使用计算机辅助精子分析(CASA)评估新鲜精子和玻璃化冷冻解冻后精子的渐进性运动能力。还进行了其他精子质量参数的检测,如欧洲鳗鲡精子的头部形态测量参数以及欧洲鲈鱼的受精能力,以测试玻璃化冷冻的效果。使解冻后运动能力最高(14±1.6%)的欧洲鲈鱼精子的玻璃化冷冻方法如下:稀释比例为1:5,使用田中稀释液,30%冷冻保护剂(15%甲醇 + 15%丙二醇),冷却装置:Cryotop,2μl液滴;欧洲鳗鲡精子的玻璃化冷冻方法为:稀释比例1:1,40%冷冻保护剂(20%甲醇和20%丙二醇),10%胎牛血清,冷却装置:Cryotop,2μl精子悬液。用玻璃化冷冻的欧洲鲈鱼精子受精产生了活胚胎(神经胚形成:2.54±1.67%)。根据ASMA分析,与新鲜精子相比,玻璃化冷冻的欧洲鳗鲡精子的头部面积和周长没有显著减小。

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