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ASSESSMENT OF BOAR SPERM VIABILITY USING A COMBINATION OF TWO FLUOROPHORES

机译:结合两种荧光评估公猪精子的活力

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A combination of the fluorophore probes, calcein acetylmethyl ester (CAM) and ethidium homodimer (EH), were used to assess viability of ejaculated boar spermatozoa. Both CAM and EH have been used as indicators of biosynthetic activity and membrane integrity in monolayer cell cultures, with CAM shown to permeate and undergo enzymatic cleavage in viable monolayer cells giving the cell a green fluorescence, and EH penetrating only membrane damaged cells giving cells a red fluorescence. To determine if these fluorophores can be used to assess boar sperm viability, ejaculates from IO boars were divided into 3 test groups (cytotoxic-treated, swim-up and washed), utilizing a split-ejaculate technique; each group consisted of both a probe-treated and control sample. Sample viability was ascertained in the control groups by visual estimation of the percentage motile spermatozoa, whereas the number of spermatozoa showing green (CAM = viable) or red (EH = non-viable) fluorescence were quantitated for each of the probe-treated groups using a fluorsecein or rhodamine filter, respectively. All spermatozoa exposed to the combined probes had an uptake of one or both fluorophores. The cytotoxic-treated group exhibited O% gross motility, with 100% of the sperm heads showing red fluorescence. In the swim-up group, no difference was detected (P>0.05) between control gross motility and the percentage of completely green fluorescing spermatozoa (85% vs. 86.6%, respectively). In the washed group, a significant difference (P=0.039) was detected between gross motility estimates and the percentage of calcein-green fluorescent spermatozoa (57% vs. 60%, respectively). This study demonstrated that 1) CAM fluoresces only viable sperm, giving off a green fluorescence, 2) EH fluoresces in only non-viable sperm, giving off a red fluorescence, 3) Visual estimation of motile sperm can approximate a semen sample's viability, but is not as precise as fluorophore determination, and 4) sperm incubation with the fluorophore combination CAM and EH provided an accurate technique for the objective assessment of boar sperm viability via their distinct fluorescent patterns in boar sperm.
机译:荧光探针,钙黄绿素乙酰甲基酯(CAM)和乙二胺均二聚体(EH)的组合用于评估射精的公猪精子的生存力。 CAM和EH均已用作单层细胞培养物中生物合成活性和膜完整性的指标,其中CAM可以渗透并在活的单层细胞中进行酶促裂解,从而使细胞发出绿色荧光,而EH仅穿透膜受损的细胞,从而使细胞获得红色荧光。为了确定这些荧光团是否可用于评估公猪精子的生存力,采用分裂射精技术将来自IO公猪的射精分为3个测试组(细胞毒素处理,游泳和洗涤)。每组均由探针处理的样品和对照样品组成。通过目测估计运动精子的百分比确定对照组的样品活力,而使用探针对每个治疗组分别定量显示绿色(CAM =存活)或红色(EH =无效)荧光的精子数量。荧光素或罗丹明过滤器。暴露于组合探针的所有精子均吸收一种或两种荧光团。细胞毒素治疗组表现出O%的总运动能力,其中100%的精子头部显示红色荧光。在游泳组中,对照组的总运动能力与发绿色荧光的精子的百分比之间没有差异(P> 0.05)(分别为85%和86.6%)。在冲洗组中,总运动估计值与钙黄绿素绿色荧光精子的百分比之间存在显着差异(P = 0.039)(分别为57%和60%)。这项研究表明1)CAM仅使活的精子发出荧光,发出绿色荧光; 2)EH仅使不活的精子发出荧光,发出红色荧光; 3)目测活动精子可以估计精液样品的活力,但是它不像荧光团测定那样精确,并且4)用荧光团CAM和EH组合进行精子孵育,可通过它们在公猪精子中不同的荧光模式为客观评估公猪精子的生存能力提供一种准确的技术。

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