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Effect of sperm dosage transportation in stallions: Effect on sperm DNA fragmentation

机译:精子剂量运输在种马中的影响:对精子DNA碎片的影响

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Artificial insemination programs for horses usually involve ex vivo handling and transporting of sperm. The present experiment was designed to: (i) assess the effect of transportation on sperm DNA integrity at different time post semen collection, and (ii) evaluate if sperm DNA quality deteriorates rapidly beyond 24 h of cooled storage. After collection, the ejaculates were extended using INRA 96 and semen was prepared for prompt analysis (A0) or 24 h/48 h cooled-shipping (B24 and C48 respectively). Each sample was assessed for sperm DNA fragmentation index (SDFI) at time 0 and after incubation for 2, 6 and 24 h at 37 degrees C. There was very little difference in SDFI between freshly extended (A0) and 24 h/48 h cooled-transported semen samples (B24/C48) at time 0. After 2 h of incubation at 37 'C, there was an increase in SDFI ranging from 2.7% to 7.5% per hour in freshly extended semen samples (A0: 5.1 +/- 1.5), while cooled-transported semen samples had a much greater increase in SDFI, ranging from 5.0% to 20.5% (B24: 14.7 +/- 5.6) and from 8.2% to 26.8% (C48: 18.3 +/- 7.2) respectively. There were not marked differences in the sperm DNA integrity between 24 and 48 h for transported samples, thus there is the possibility of desirable fertility with use of stallion sperm after 48 h of cooled storage.
机译:用于马匹的人工授精计划通常涉及前体内处理和运输精子。本实验设计为:(i)评估在精液收集后不同时间对不同时间的精子DNA完整性的运输的影响,(ii)如果精子DNA质量迅速降低24小时,则评估冷却储存的24小时。在收集后,使用在ARS 96和分别用于及时分析(A0)或24H / 48 H冷却的(B24和C48)进行射精进行eJAculate。在37摄氏度温育2,6和24小时的时间内评估每个样品的精子DNA碎片指数(SDFI),在37℃下孵育2,6和24小时。在新鲜延伸(A0)和24h / 48小时之间的SDFI差异很小 - 在37'c孵育2小时后,SDFI在新延长的精液样本中增加了2小时后,SDFI的增加(A0:5.1 +/- 1.5),虽然冷却的转运的精液样品在SDFI中增加了更大的增加,但分别为5.0%至20.5%(B24:14.7 +/- 5.6),分别为8.2%至26.8%(C48:18.3 +/- 7.2) 。对于运输样品,24至48小时的精子DNA完整性没有明显的差异,因此在冷却储存48小时后使用马氏精子的使用具有所需的生育能力。

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