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Seminal plasma applied post-thawing affects boar sperm physiology: A flow cytometry study

机译:解冻后应用精浆对公猪精子生理的影响:流式细胞术研究

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Cryopreservation induces extensive biophysical and biochemical changes in the sperm. In the present study, we used flow cytometry to assess the capacitation-like status of frozen-thawed boar spermatozoa and its relationship with intracellular calcium, assessment of membrane fluidity, modification of thiol groups in plasma membrane proteins, reactive oxygen species (ROS) levels, viability, acrosomal status, and mitochondrial activity. This experiment was performed to verify the effect of adding seminal plasma on post-thaw sperm functions. To determine these effects after cryopreservation, frozen-thawed semen from seven boars was examined after supplementation with different concentrations of pooled seminal plasma (0%, 10%, and 50%) at various times of incubation from 0 to 4 hours. Incubation caused a decrease in membrane integrity and an increase in acrosomal damage, with small changes in other parameters (P > 0.05). Although 10% seminal plasma showed few differences with 0% (ROS increase at 4 hours, P < 0.05), 50% seminal plasma caused important changes. Membrane fluidity increased considerably from the beginning of the experiment, and ROS and free thiols in the cell surface increased by 2 hours of incubation. By the end of the experiment, viability decreased and acrosomal damage increased in the 50% seminal plasma samples. The addition of 50% of seminal plasma seems to modify the physiology of thawed boar spermatozoa, possibly through membrane changes and ROS increase. Although some effects were detrimental, the stimulatory effect of 50% seminal plasma could favor the performance of post-thawed boar semen, as showed in the field (Garcia JC, Dominguez JC, Pena FJ, Alegre B, Gonzalez R, Castro MJ, Habing GG, Kirkwood RN. Thawing boar semen in the presence of seminal plasma: effects on sperm quality and fertility. Anim Reprod Sci 2010;119:160-5).
机译:冷冻保存可引起精子发生广泛的生物物理和生化变化。在本研究中,我们使用流式细胞仪评估冻融的公猪精子的获能状态,及其与细胞内钙的关系,评估膜的流动性,修饰质膜蛋白中的硫醇基团,活性氧(ROS)水平,生存能力,顶体状态和线粒体活性。进行该实验以验证添加精浆对解冻后精子功能的影响。为了确定冷冻保存后的这些作用,在0至4小时的不同孵育时间中,补充了不同浓度的混合精浆(0%,10%和50%)后,检查了7只公猪的冻融精液。孵化导致膜完整性下降和顶体损伤增加,其他参数变化很小(P> 0.05)。尽管10%的精浆与0%的差异很小(4小时ROS增加,P <0.05),但50%的精浆引起了重要的变化。从实验开始起,膜的流动性显着增加,孵育2小时后,细胞表面的ROS和游离硫醇增加。到实验结束时,在50%的精浆血浆样品中,活力降低,顶体损伤增加。添加50%的精浆似乎可以改变被融化的公猪的精子的生理,可能是通过膜的变化和ROS的增加。尽管有些影响是有害的,但如田间试验所示,50%精浆的刺激作用可能有助于解冻后的公猪精液的表现(Garcia JC,Dominguez JC,Pena FJ,Alegre B,Gonzalez R,Castro MJ,Habing GG,Kirkwood RN。在精浆存在下解冻公猪精液:对精子质量和生育力的影响。Anim Reprod Sci 2010; 119:160-5)。

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