Luther I, Jakop U, Lueders I, Tordiffe A, Franz C, Schiller J, Kotze A, Müller K
Research & Scientific Services, National Zoological Gardens of South Africa, Pretoria, South Africa.
Department of Reproductive Biology, Leibniz Institute for Zoo and Wildlife Research, Berlin, Germany.
Theriogenology. 2017 Feb;89:295-304. doi: 10.1016/j.theriogenology.2016.10.024. Epub 2016 Nov 9.
Optimizing cryopreservation protocols for nondomestic felids contributes to the successful development of assisted reproduction techniques and genetic resource banking. In this study, we describe a simple cryopreservation procedure for African lion (Panthera leo) ejaculates, which was tested with different packaging options and different sperm numbers per dose. By applying urethral catheterization and electroejaculation, 17 ejaculates with greater than 20% motile and greater than 5% progressively motile sperm were collected. A lyophilized extender (a modified egg yolk-Tes-Tris-fructose-glycerol medium) was rehydrated and added in one step at ambient temperature (∼25 °C) to semen, which was prediluted in cell culture medium M199. After slow cooling of insulated samples to 15 °C in a refrigerator (4 °C), the samples were fast frozen over the surface of liquid nitrogen or in a dry shipper. Aliquots of 300 μL containing 20 × 10 sperm were frozen in cryovials and in 0.5-mL straws. Differences were observed in the total motility after thawing between vial (31.5 ± 14.1%) and straw freezing (20.1 ± 8.6%). However, the subpopulations of vital (22.7 ± 7.8% for vial and 19.8 ± 8.5% for straw) and progressively motile (10.0 ± 7.9% for vial and 10.0 ± 6.4% for straw) sperm after washing and 1 hour incubation at 38 °C were of similar magnitude, velocity, and linearity for both packaging options. After freezing of five ejaculates with 20, 60, and 100 × 10 sperm per dose, best results were achieved at the lowest concentration. In general, post-thaw results were highly variable (2.2% and 56.5% total motility) and not correlated to motility or morphology of the fresh semen. To further characterize semen quality, we assessed the protective potential of seminal fluid against oxidative stress, which might be challenged on freeze thawing. The capacity of seminal fluid to reduce radicals was measured in 10 semen samples by electron spin resonance spectroscopy and a spin-labeled fatty acid as a radical probe. Moreover, we determined the lysophosphatidylcholines (LPC) as potential lipid oxidation products in the sperm and erythrocytes of the males. Individuals with a high radical reduction capacity in the seminal fluid and a low LPC content in their erythrocytes showed a better cryosurvival of sperm. This is a first indication that seminal fluid may affect the freezing potential of African lion ejaculates.
优化非家养猫科动物的冷冻保存方案有助于辅助生殖技术和遗传资源库的成功发展。在本研究中,我们描述了一种针对非洲狮(Panthera leo)精液的简单冷冻保存程序,该程序在不同包装选项和每剂量不同精子数量下进行了测试。通过应用尿道插管和电刺激采精,收集到了17份精液,其中活动精子大于20%且进行性活动精子大于5%。将一种冻干的稀释液(一种改良的蛋黄 - Tes - Tris - 果糖 - 甘油培养基)复水,并在室温(约25°C)下一次性加入到预先在细胞培养基M199中稀释的精液中。在冰箱(4°C)中将保温样品缓慢冷却至15°C后,将样品在液氮表面或干式运输箱中快速冷冻。将含有20×10⁶精子的300μL等分试样分别冷冻在冻存管和0.5mL细管中。观察到解冻后冻存管(31.5±14.1%)和细管冷冻(20.1±8.6%)的总活力存在差异。然而,在38°C洗涤并孵育1小时后,两种包装方式下有活力精子亚群(冻存管为22.7±7.8%,细管为19.8±8.5%)和进行性活动精子亚群(冻存管为10.0±7.9%,细管为10.0±6.4%)的数量、速度和线性相似。在每剂量分别含有20×10⁶、60×10⁶和100×10⁶精子的5份精液冷冻后,最低浓度时取得了最佳结果。总体而言,解冻后的结果差异很大(总活力为2.2%和56.5%),且与新鲜精液的活力或形态无关。为了进一步表征精液质量,我们评估了精液对氧化应激的保护潜力,氧化应激可能在冻融过程中受到挑战。通过电子自旋共振光谱法和使用自旋标记脂肪酸作为自由基探针,在10份精液样本中测量了精液还原自由基的能力。此外,我们测定了雄性精子和红细胞中潜在的脂质氧化产物溶血磷脂酰胆碱(LPC)。精液中自由基还原能力高且红细胞中LPC含量低的个体,其精子的冷冻存活率更高。这首次表明精液可能会影响非洲狮精液的冷冻潜力。
