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使用精子-透明质酸结合试验评估单峰驼精子质量。

Use of a sperm-Hyaluronan binding assay for evaluation of sperm quality in dromedary camels.

机构信息

Swedish University of Agricultural Sciences, Department of Clinical Sciences, Sweden.

Institute for Health Research Aragón (IIS Aragón), Zaragoza 50009, Spain.

出版信息

Anim Reprod Sci. 2024 Nov;270:107596. doi: 10.1016/j.anireprosci.2024.107596. Epub 2024 Sep 8.

Abstract

The objective of this study was to assess the ability of camel spermatozoa to bind in the Hyaluronan Binding Assay (HBA), to determine if conventional sperm quality parameters, in vitro fertilization capacity, and precursor of A-Kinase Anchoring Protein 4 (proAKAP4) values correlate with HBA results. The potential to predict post-thaw fertilization performance from HBA for fresh dromedary camel sperm was also evaluated. Semen samples were collected and assessed both fresh and post thawing, at 0 h and 1.5 h. Conventional semen analysis, HBA, and a proAKAP4 biomarker-test were used to validate sperm quality. A heterologous sperm penetration assay using zona pellucida-free goat oocytes was used to assess in vitro sperm fertilizing capacity. The results showed that dromedary camel spermatozoa bound to hyaluronan with no correlation between results from fresh samples and after thawing. Furthermore, the proAKAP4 test results showed a negative correlation with HBA at 0 h after thawing (r = - 0.62; P = 0.03). In the conventional analysis, only progressive motility (r = 0.65; P = 0.02) and straightness correlated with HBA for fresh semen (r = 0.69; P = 0.01). In the sperm penetration assay, a moderate but non-significant correlation was identified between fresh sperm HBA and penetration (r = 0.52; P = 0.07). In conclusion, results suggested that HBA can be used to assess camel sperm properties, but further investigation is needed to understand its correlation with other sperm quality parameters. The HBA score from fresh dromedary camel sperm was unable to predict post-thaw fertilization performance.

摘要

本研究旨在评估骆驼精子在透明质酸结合试验(HBA)中的结合能力,确定常规精子质量参数、体外受精能力和 A 激酶锚定蛋白 4 前体(proAKAP4)值是否与 HBA 结果相关。还评估了从 HBA 预测新鲜骆驼精子解冻后受精性能的潜力。收集精液样本并在新鲜和解冻后 0 h 和 1.5 h 进行评估。使用常规精液分析、HBA 和 proAKAP4 生物标志物测试来验证精子质量。使用无透明带的山羊卵母细胞进行异源精子穿透试验来评估体外精子受精能力。结果表明,骆驼精子与透明质酸结合,新鲜样本和解冻后样本的结果之间没有相关性。此外,解冻后 0 h 的 proAKAP4 测试结果与 HBA 呈负相关(r = - 0.62;P = 0.03)。在常规分析中,只有前向运动(r = 0.65;P = 0.02)和直线度与新鲜精液的 HBA 相关(r = 0.69;P = 0.01)。在精子穿透试验中,新鲜精子 HBA 与穿透之间存在中度但无统计学意义的相关性(r = 0.52;P = 0.07)。总之,结果表明 HBA 可用于评估骆驼精子特性,但需要进一步研究以了解其与其他精子质量参数的相关性。新鲜骆驼精子的 HBA 评分无法预测解冻后的受精性能。

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