流式细胞术比较游泳和Percoll梯度技术分离冻融人精子的效果。

International Journal of Fertility Pub Date : 1992-09-01
Y Chen, M S Obhrai, J Chapman, J L Cuthbert, A Williams, L Tang
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引用次数: 0

摘要

采用游泳法和Percoll密度梯度法对冷冻后的活精子进行了分离,并与新鲜精子的细胞表面寡糖成分进行了比较。精子用FITC-Con A标记,荧光显微镜和流式细胞术分析。在荧光显微镜下,仅在颈部区域均匀标记新鲜精子。通过游泳或Percoll密度梯度获得的冻融精子显示出两种染色模式:一种精子种群仅在颈部区域染色,而另一种精子种群在颈部和顶体区域均染色。两种技术回收的精子之间没有明显的差异。新鲜精子的流式细胞仪显示单峰荧光,而冷冻保存的精子有两个荧光峰。通过Percoll密度梯度回收的样本中含有与新鲜精子相同的荧光模式的精子数量明显多于通过游泳回收的精子。低温保存改变了精子细胞表面的寡糖成分。通过Percoll密度梯度恢复冷冻保存的精子产生比游泳更大比例的类似新鲜精子的精子。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Flow cytometric comparison between swim-up and Percoll gradient techniques for the separation of frozen-thawed human spermatozoa.

Viable human spermatozoa were recovered from cryopreservation by either swim-up or Percoll density gradient techniques and their cell-surface oligosaccharide components were compared to those of fresh sperm. Sperm were labeled with FITC-Con A and analyzed by fluorescence microscopy and flow cytometry. By fluorescence microscopy, fresh sperm were uniformly labeled in the neck region alone. Frozen-thawed sperm, obtained by either swim-up or Percoll density gradients, showed two patterns of staining: one sperm population was stained in the neck region only, whilst another showed staining in both the neck and acrosome regions. No difference between sperm recovered by the two techniques was apparent. Flow cytometry profiles of fresh sperm revealed a single peak of fluorescence, whereas cryopreserved sperm gave two peaks of fluorescence. Samples recovered by Percoll density gradient contained significantly more sperm with the same fluorescence pattern as that observed for fresh sperm than did those recovered by swim-up. Cryopreservation alters the cell-surface oligosaccharide components of spermatozoa. Recovery of cryopreserved sperm by Percoll density gradient yields a greater proportion of sperm which resemble fresh sperm than does swim-up.

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