首页> 外文期刊>Theriogenology >A pilot study on post-thawing quality of Iberian red deer spermatozoa (epididymal and electroejaculated) depending on glycerol concentration and extender osmolality
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A pilot study on post-thawing quality of Iberian red deer spermatozoa (epididymal and electroejaculated) depending on glycerol concentration and extender osmolality

机译:伊比利亚马鹿精子(附睾和电射精)解冻后质量的初步研究,具体取决于甘油浓度和体质渗透压

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The optimization of cryopreservation extenders is a fundamental issue for adequately performing germplasm banking on wild species. We have tested two glycerol concentrations (4 and 8%), and three extender osmolalities (320, 380 and 430 mOsm/kg; before adding cryoprotectants), for cryopreservation of epididymal and ejaculated sperm samples from Iberian red deer. All the extenders were based on Tes-Tris and fructose (for osmolality adjustment), and complemented with 20% egg yolk. Epididymal and ejaculated sperm samples were obtained from the cauda epididymis (post-mortem) and using electroejaculation, respectively. Samples were diluted 1:1 with each extender and equilibrated for 2 h at 5 degrees C. Then, they were diluted down to 100x10(6) sperm/mL and frozen at -20 degrees C/min. Post-thawed samples were assessed for motility (CASA), HOS test, proportion of swollen (osmotically challenged) cells in the untreated sample, viability and acrosomal status. For epididymal samples, 8% glycerol rendered a slightly higher proportion of intact acrosomes on viable spermatozoa than 4%; regarding extender osmolality, 380 and 430 mOsm/kg rendered higher motility results, and the 430 mOsm/kg yielded the lowest proportion of swollen spermatozoa. For ejaculated samples, 4% glycerol yielded more viable spermatozoa than 8%; for extender osmolality, 320 mOsm/kg rendered the highest percentages of progressively motile and viable spermatozoa, although 380 mOsm/kg extender was not significantly different. These results show that sample source influences extender suitability, and that extenders should be isoosmotic or rather slightly hyperosmotic. Future studies should test multiple glycerol concentrations and extender osmolalities in order to adjust them to these kinds of sample.
机译:低温保存扩展剂的优化是在野生物种上充分执行种质库的基本问题。我们已经测试了两种甘油浓度(分别为4%和8%)和三种增量剂同渗容摩尔浓度(320、380和430 mOsm / kg;在添加冷冻保护剂之前),用于冷冻保存伊比利亚马鹿的附睾和射精精子样品。所有增量剂均基于Tes-Tris和果糖(用于渗透压调节),并辅以20%的蛋黄。附睾和射精的精子样本分别来自附睾马尾(验尸)和使用电射精。用每种增量剂按1:1稀释样品,并在5摄氏度下平衡2小时。然后将其稀释至100x10(6)精子/毫升,并在-20摄氏度/分钟下冷冻。评估解冻后样品的运动性(CASA),HOS测试,未处理样品中溶胀(渗透压)细胞的比例,生存力和顶体状态。对于附睾样品,8%的甘油使完整的顶体在活精子上的比例略高于4%;就增量渗透压而言,380和430 mOsm / kg的运动性结果更高,而430 mOsm / kg的精子肿胀率最低。对于射精的样品,4%的甘油比8%产生更多的活精子。对于增量剂的渗透压,尽管380 mOsm / kg的增量剂无显着差异,但320 mOsm / kg的比例能使运动精子和存活精子的比例最高。这些结果表明,样品来源会影响扩展剂的适用性,并且扩展剂应该是等渗的,或者应该是高渗的。未来的研究应测试多种甘油浓度和增量渗透压,以便将它们调整为适合此类样品。

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