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Different functional states of ram spermatozoa analysed by partition in an aqueous two-phase system

机译:两相水系统中分配作用分析精子的不同功能状态

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The surface of spermatozoa plays a critical role in man stages involved in fertilisation. The plasma membrane undergoes important alterations in the male and female reproductive tract, which result in the ability of spermatozoa to fertilise eggs. One of these membrane modifications is sperm capacitation, a process by which sperm interacts with the zona pellucida receptors leading to the acrosome reaction. It has been proposed that the freezing process induces capacitation-like changes to spermatozoa, and that this premature capacitation could explain the reduction in longevity and fertilising capacity of cryopreserved mammalian spermatozoa. Our research focused on the relationship between membrane alterations occurring throughout freezing-thawing and the processes of capacitation and acrosome reaction. We used centrifugal countercurrent distribution (CCCD) analysis to compare the partition behaviour of ram spermatozoa that was either subjected to cold-shock or frozen-thawed wit capacitated and acrosome reacted samples. In addition, the effect of the induced acrosome reaction on membrane integrity of ram spermatozoa was studied using biochemical markers and electron microscopy scanning. The CCCD analysis revealed important similarities between the surface characteristics of capacitated and cold-shocked sperm as well as between acrosome-reacted and frozen-thawed sperm. Cold-shocked and capacitated sperm showed an increased cell affinity for the lower dextran-rich phase as well as a decreased heterogeneity. Likewise, the induction of the acrosome reaction resulted in a loss of viability and an important decrease in cell surface heterogeneity compared to the untreated-control sample. Similar surface changes were found when semen samples were frozen with either Fiser or milk-yolk extender. These results confirm those obtained for membrane integrity by fluorescence markers. Thus, the high cell viability value found in the control sample (74.5%) was greatly decreased after cold-shock (22.2%), cryopreservation (26.38% Fiser medium, 24.8% milk-yolk medium) and acrosome reaction (6.6%), although it was preserved after inducing capacitation (46.7%). The study using electron microscopy scanning revealed dramatic structural alterations provoked by the induction of the acrosome reaction.
机译:精子的表面在受精过程中起着至关重要的作用。质膜在雄性和雌性生殖道中发生重要变化,从而导致精子使卵子受精的能力。这些膜的修饰之一是精子获能,即精子与透明带受体相互作用导致顶体反应的过程。已经提出,冷冻过程引起精子获能的改变,并且这种过早的获能可以解释低温保存的哺乳动物精子的寿命和受精能力的降低。我们的研究集中在整个冻融过程中发生的膜变化与获能和顶体反应过程之间的关系。我们使用离心逆流分布(CCCD)分析来比较受精子和顶体反应的冷激或冷冻融化的精子在精子中的分配行为。此外,使用生化标记和电子显微镜扫描研究了诱导的顶体反应对公羊精子膜完整性的影响。 CCCD分析揭示了获能的和冷激的精子的表面特征之间以及顶体反应的和冻融的精子之间的重要相似性。冷休克和获能的精子对低葡聚糖富集相的细胞亲和力增加,异质性降低。同样,与未处理的对照样品相比,顶体反应的诱导导致活力的丧失和细胞表面异质性的显着降低。当精子样品用Fiser或乳黄增量剂冷冻时,发现相似的表面变化。这些结果证实了通过荧光标记获得的膜完整性的结果。因此,在冷休克(22.2%),冷冻保存(26.38%Fiser培养基,24.8%乳黄培养基)和顶体反应(6.6%)之后,对照样品(74.5%)中发现的高细胞活力值大大降低,尽管诱导后仍能保留(46.7%)。使用电子显微镜扫描的研究表明,顶体反应的诱导引起了显着的结构改变。

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