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Damage assessment of the equine sperm membranes by fluorimetric technique.

机译:用荧光技术评估马精子膜的损伤。

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摘要

To validate a practical technique of simultaneous evaluation of the plasma, acrosomal and mitochondrial membranes in equine spermatozoa three fluorescent probes (PI, FITC-PSA and MITO) were associated. Four ejaculates from three stallions (n=12) were diluted in TALP medium and split into 2 aliquots, 1 aliquot was flash frozen in liquid nitrogen to induce damage in cellular membranes. Three treatments were prepared with the following fixed ratios of fresh semen: flash frozen semen: 100:0 (T100), 50:50 (T50), and 0:100 (T0). A 150- micro L aliquot of diluted semen of each treatment was added of 2 micro L of PI, 2 micro L of MITO and 80 micro L of FITC-PSA; incubated at 38.5 degrees C/8 min, and sperm cells were evaluated by epifluorescent microscopy. Based in regression analysis, this could be an efficient and practical technique to assess damage in equine spermatozoa, as it was able to determine the sperm percentage more representative of the potential to fertilize the oocyte.
机译:为了验证同时评估血浆,马精子中顶体膜和线粒体膜的实用技术,需要结合三种荧光探针(PI,FITC-PSA和MITO)。在TALP培养基中稀释来自3种公马(n = 12)的4种射精,分成2等分试样,将1等分试样在液氮中速冻,以诱导细胞膜损伤。用以下固定比例的新鲜精液制备三种处理:速冻精液:100:0(T100),50:50(T50)和0:100(T0)。每次处理均加入150微升稀释精液的等分试样,其中包括2微升PI,2微升MITO和80微升FITC-PSA;在38.5℃/ 8分钟温育,并通过落射荧光显微镜评估精子细胞。基于回归分析,这可能是评估马精子中损伤的有效且实用的技术,因为它能够确定更能代表卵母细胞受精潜力的精子百分比。

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