The effects of co-culture of human spermatozoa with human immortalized endometrial cells - epithelial or stromal - on sperm movement characteristics, including hyperactivation, were studied using computer-assisted sperm analysis (CASA). Epithelial and stromal cell types could be separated following 8-10 days of culture of endometrial cells originating from human biopsies. Both cell types were immortalized by the SV 40 large T antigen. Co-incubation of sperm with epithelial and stromal monolayers enhanced the rate of hyperactivation24.9% (P <0.05) and 17.8% (P = 0.05) versus 9.5% as control, respectively, whereas the majority of motility parameters remained unchanged. Conditioned media had no effect upon sperm parameters, including hyperactivation. Co-incubation with either monolayer was able to maintain sperm motility over a longer period than incubation in control medium alone.

In four patients whose spermatozoa did not exhibit hyperactivation, co-incubation with epithelial cells, but not conditioned medium, allowed normal rates of hyperactivation (range6.9-15.6%).

译文

使用计算机辅助精子分析(CASA)研究了人类精子与人类永生化子宫内膜细胞-上皮或基质共培养对精子运动特征(包括过度活化)的影响。在培养源自人类活组织检查的子宫内膜细胞8-10天后,可以分离上皮和基质细胞类型。两种细胞类型都可以通过SV 40大T抗原获得永生。将精子与上皮和基质单层共同孵育可提高超活化率,分别为对照组的24.9%(P <0.05)和17.8%(P = 0.05),而对照组为9.5%,而大多数运动参数保持不变。条件培养基对精子参数没有影响,包括过度激活。与单独在对照培养基中孵育相比,与任一单层一起共同孵育能够在更长的时间内维持精子活力。

在四名精子未表现出过度激活的患者中,与上皮细胞共同孵育,但不与条件培养基共同孵育,允许正常的过度激活率(范围6.9-15.6%)。

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