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首页> 外文期刊>Theriogenology >DNA integrity of canine spermatozoa during chill storage assessed by the sperm chromatin dispersion test using bright-field or fluorescence microscopy
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DNA integrity of canine spermatozoa during chill storage assessed by the sperm chromatin dispersion test using bright-field or fluorescence microscopy

机译:通过明场或荧光显微镜通过精子染色质分散测试评估犬冷库中DNA的完整性

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The objective of this study was to evaluate the effect of chill storage on canine sperm DNA fragmentation assessed by the sperm chromatin dispersion test using bright-field microscopy with Wright solution (sDF-B) or fluorescence microscopy with propidium iodide (sDF-F). The relationship and agreement between the results obtained with both staining methods were analyzed. The values of DNA fragmentation indexes (sDF-F and sDF-B) were compared at each time of chill storage (0, 24, 48, 72, and 96 hours). Additionally, the sperm DNA fragmentation rate (slope) was compared between the methods during chill storage. Good agreement and no significant differences between values obtained with both staining procedures were observed. Finally, the effect of chill storage for up to 96 hours was assessed on sperm motility parameters and DNA fragmentation indexes. Significant differences were found after 48 hours of chill storage, obtaining greater values of fragmented DNA. Progressive sperm motility was lower just after 96 hours of chill storage, and no effect was found in total sperm motility. In conclusion, the Sperm-Halomax kit, developed for canine semen and based on the sperm chromatin dispersion test, can be used accurately under bright-field or fluorescence microscopy to assess the sperm DNA integrity of canine semen during chill storage. The sperm DNA fragmentation index increased after 48 hours of chill storage, thereby detecting sperm damage earlier than other routine sperm parameters, such as sperm motility. (C) 2015 Elsevier Inc. All rights reserved.
机译:这项研究的目的是评估冷冻保存对犬精子DNA片段化的影响,该片段是通过使用Wright溶液的明场显微镜(sDF-B)或使用碘化丙啶(sDF-F)的荧光显微镜通过精子染色质分散测试评估的。分析了两种染色方法获得的结果之间的关系和一致性。在每次冷藏时(0、24、48、72和96小时)比较DNA片段化指数(sDF-F和sDF-B)的值。另外,比较了冷冻保存过程中两种方法之间的精子DNA片段化率(斜率)。观察到良好的一致性,并且在两种染色方法中获得的值之间均未观察到明显差异。最后,对精子活力参数和DNA碎片指数评估了冷藏长达96小时的效果。冷藏48小时后发现显着差异,获得了更大的片段化DNA值。冷藏96小时后,进行性精子活动性降低,总精子活动性没有影响。总之,基于精子染色质分散测试开发的用于犬精液的Sperm-Halomax试剂盒可在明亮视野或荧光显微镜下准确用于评估冷冻保存过程中犬精液的DNA完整性。冷藏48小时后,精子DNA碎片指数增加,从而比其他常规精子参数(例如精子活力)更早地检测出精子损伤。 (C)2015 Elsevier Inc.保留所有权利。

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