寻找公牛精子质量与ESR1基因多态性的关系

E. Nikitkina, A. Musidray, S. Bogdanova, A. Krutikova
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摘要

材料和方法。在OJSC Nevskoe收集了53头公牛的精液。对110份公牛精液样本进行了分析。使用Argus-CASA (ArgusSoft,俄罗斯)测定精子质量。膜的完整性是用黑芥子-伊红染料(Diam,俄罗斯)和Motic ba410显微镜染色来测定的。使用Expert-001仪器测定精子呼吸。能量系统的功能状态通过添加呼吸解耦剂和磷酸化2,4二硝基苯酚(2,4- dnf)的呼吸反应来评估。用苯酚-氯仿法从精液中分离出用于遗传分析的DNA。Sanger测序在Applied Biosystems 3500基因分析仪上进行,使用商用BigDye®Terminator v3.1测序标准试剂盒(Applied Biosystems),按照制造商的协议。精子质量具有高度的个体差异。由此可见,射精体积为2 ~ 15ml,精子浓度为6 ~ 17亿个/ml,射精中精子总数为16 ~ 150亿个,进行性运动率为0 ~ 85%。ESR1基因鉴定出4个snp。除ESR1 665 G>C与精子浓度和顶体肿胀数量显著相关外,ESR1基因多态性未发现显著相关
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Search for associations of bull sperm quality with ESR1 gene polymorphism
Materials and methods. The semen of 53 bulls was collected at OJSC Nevskoe. A total of 110 bull semen samples were analyzed. Sperm quality was determined using Argus-CASA (ArgusSoft, Russia). Membrane integrity was determined by staining the samples with nigrosine-eosin dye (Diam, Russia) and a Motic BA 410 microscope. Spermatozoa respiration was determined using an Expert-001 instrument. The functional state of the energy system was assessed by the reaction of respiration to the addition of the uncoupler of respiration and phosphorylation, 2,4 dinitrophenol (2,4-DNF). DNA for genetic analysis was isolated from semen by the phenol-chloroform method. Sanger sequencing was performed on an Applied Biosystems 3500 Genetic Analyzer using commercial BigDye® Terminator v3.1 Sequencing Standard Kits (Applied Biosystems) according to the manufacturer's protocol.Results. Sperm quality were characterized by high individual variability. Thus, the volume of the ejaculate was from 2 to 15 ml, the concentration of spermatozoa was from 0.6 to 1.7 billion/ml, the total number of spermatozoa in the ejaculate was from 1.6 to 15 billion, and progressive motility was from 0 to 85%. Four SNPs were identified for the ESR1 gene. No significant associations of ESR1 gene polymorphism were found, except for a significant association of ESR1 665 G>C with spermatozoa concentration and the number of swollen acrosomes
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