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不同冷冻保护剂对公牛精子质量、DNA 完整性和氧化应激参数的影响。

Effects of various cryoprotectants on bull sperm quality, DNA integrity and oxidative stress parameters.

机构信息

Livestock Central Research Institute, Lalahan, Ankara, Turkey.

出版信息

Cryobiology. 2013 Feb;66(1):38-42. doi: 10.1016/j.cryobiol.2012.10.006. Epub 2012 Nov 10.

Abstract

The objectives of this study was to compare the effects of type and concentration of cryoprotectants glycerol (G), ethylene glycol (EG) and dimethyl sulfoxide (DMSO) on the plasma membrane and DNA integrity as well as antioxidant activity of cryopreserved Eastern Anatolian red bull sperm. Ejaculates were collected from the three bulls using an artificial vagina twice a week. The ejaculates were pooled to increase the semen volume for replication and to eliminate variability among the evaluated samples. The pooled ejaculates were also split into seven equal experimental groups and diluted with the modified base extender to a final spermatozoa concentration of 15×10(6)/ml. The extended samples were cooled slowly to 4°C and equilibrated for 4h. They were then loaded into 0.25ml French straws and frozen using a digital freezing machine at 3 programmed rates: -3°C/min from +4°C to -10°C, -40°C/min from -10°C to -100°C, and -20°C/min from -100°C to -140°C. Thereafter, the straws were plunged into liquid nitrogen at -196°C. Frozen straws were thawed individually at 37°C for 30s in a water bath to analyse progressive motility and sperm motion characteristics as well as membrane integrity using hypo-osmotic swelling test. Biochemical assays were performed in a spectrophotometer using commercial kits. DNA damage was evaluated by Comet Assay using Image Analysis System. 6% G exhibited the greatest percentages of CASA (43.7±2.92%) and progressive (26.4±2.64%) motilities when compared to the other groups (P<0.001). 6% G and 6% EG showed the greatest values of preserved membrane integrity (P<0.001). 6% DMSO and 3% EG + 3% DMSO resulted in greater chromatin damage than the other groups (P<0.001). The antioxidant activities of GPx, GSH, and CAT as well as the total antioxidant activity were affected by the type of cryoprotectant; notably, 2% G+2% EG+2% DMSO yielded the lowest activities when compared to the other groups (P<0.001). In conclusion, no advantages were found in using EG or DMSO to replace G in bull sperm cryopreservation. Freezing with cryoprotectant 6% G yielded the best post-thaw sperm characteristics for Eastern Anatolian Red bull spermatozoa.

摘要

本研究的目的是比较甘油(G)、乙二醇(EG)和二甲基亚砜(DMSO)三种不同类型和浓度的抗冻剂对冷冻保护后精子质膜和 DNA 完整性以及抗氧化活性的影响。采用人工授精法每周从三头公牛中采集两次精液。将采集的精液混合以增加精液量进行复制,并消除评估样本之间的差异。将混合的精液分成七个相等的实验组,并用改良的基础稀释液稀释至最终精子浓度为 15×10(6)/ml。将扩展的样品缓慢冷却至 4°C 并平衡 4 小时。然后将它们装入 0.25ml 法国 straws 中,并使用数字冷冻机以 3 种编程速度冷冻:从+4°C 到-10°C 为-3°C/min,从-10°C 到-100°C 为-40°C/min,从-100°C 到-140°C 为-20°C/min。之后, straws 立即浸入-196°C 的液氮中。将冷冻 straws 在 37°C 的水浴中单独解冻 30 秒,以分析在低渗肿胀试验中的前向运动和精子运动特性以及质膜完整性。使用商业试剂盒在分光光度计中进行生化分析。通过 Comet 分析使用图像分析系统评估 DNA 损伤。与其他组相比(P<0.001),6% G 显示出最高百分比的 CASA(43.7±2.92%)和前向运动(26.4±2.64%)。6% G 和 6% EG 显示出最高的质膜完整性保留值(P<0.001)。3% EG+3% DMSO 和 6% DMSO 导致比其他组更大的染色质损伤(P<0.001)。GPx、GSH 和 CAT 的抗氧化活性以及总抗氧化活性受到抗冻剂类型的影响;值得注意的是,与其他组相比,2% G+2% EG+2% DMSO 产生的活性最低(P<0.001)。总之,在牛精子冷冻保存中使用 EG 或 DMSO 代替 G 没有发现优势。使用 6% G 冷冻保护剂冷冻可获得东方安纳托利亚红牛精子解冻后最佳的精子特性。

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