Involvement of Ca2+-ATPase in suppressing the appearance of bovine helically motile spermatozoa with intense force prior to cryopreservation

Duritahala, M. Sakase, H. Harayama
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引用次数: 2

Abstract

In cattle, cryopreserved spermatozoa are generally used for artificial insemination (AI). Many of these specimens exhibit helical movement, although the molecular mechanisms underlying this phenomenon remain unclear. This study aimed to characterize helically motile spermatozoa, investigate the involvement of Ca2+-ATPase in suppressing the appearance of these spermatozoa prior to cryopreservation, and examine the potential of helical movement as an index of sperm quality. In the cryopreserved semen, approximately 50% of spermatozoa were helically motile, whereas approximately 25% were planarly motile. The helically motile samples swam significantly faster than those with planar movement, in both non-viscous medium and viscous medium containing polyvinylpyrrolidone. In contrast, in non-cryopreserved semen, planarly motile spermatozoa outnumbered those that were helically motile. Fluorescence microscopy with Fluo-3/AM and propidium iodide showed that flagellar [Ca2+]i was significantly higher in cryopreserved live spermatozoa than in non-cryopreserved live ones. The percentage of non-cryopreserved helically motile spermatozoa was approximately 25% after washing, and this increased significantly to approximately 50% after treatment with an inhibitor of sarcoplasmic reticulum Ca2+-ATPases (SERCAs), “thapsigargin.” Immunostaining showed the presence of SERCAs in sperm necks. Additionally, the percentages of cryopreserved helically motile spermatozoa showed large inter-bull differences and a significantly positive correlation with post-AI conception rates, indicating that helical movement has the potential to serve as a predictor of the fertilizing ability of these spermatozoa. These results suggest that SERCAs in the neck suppress the cytoplasmic Ca2+-dependent appearance of helically motile spermatozoa with intense force in semen prior to cryopreservation.
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参与Ca2+- atp酶在抑制牛螺旋运动精子的外观与强力之前冷冻保存
在牛中,冷冻保存的精子通常用于人工授精(AI)。这些标本中的许多都表现出螺旋运动,尽管这种现象背后的分子机制尚不清楚。本研究旨在描述螺旋运动精子的特征,研究Ca2+- atp酶在冷冻保存前抑制这些精子外观的作用,并研究螺旋运动作为精子质量指标的潜力。在冷冻保存的精液中,大约50%的精子是螺旋运动的,而大约25%是平面运动的。无论在无粘性介质中还是在含有聚乙烯吡咯烷酮的粘性介质中,螺旋运动样品的游动速度都明显快于平面运动样品。相比之下,在非冷冻保存的精液中,平面运动精子的数量超过螺旋运动精子的数量。荧光显微镜和碘化丙啶显示,冷冻保存的活精子鞭毛[Ca2+]i明显高于非冷冻保存的活精子。洗涤后,非冷冻保存的螺旋运动精子的百分比约为25%,在用肌浆网Ca2+- atp酶(SERCAs)抑制剂“thapsigarin”治疗后,这一比例显着增加到约50%。免疫染色显示精子颈部存在SERCAs。此外,冷冻保存的螺旋运动精子的百分比显示出很大的公牛间差异,并与人工智能后受孕率显著正相关,这表明螺旋运动有可能作为这些精子受精能力的预测指标。这些结果表明,颈部的SERCAs在冷冻保存前强烈地抑制了精子中螺旋运动精子的细胞质Ca2+依赖性外观。
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