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An improved efficient method for analyzing human sperm chromosomes using zona-free hamster ova.

机译:一种改进的有效的方法使用不含透明带的仓鼠卵来分析人的精子染色体。

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摘要

We have developed an improved method for analyzing human sperm chromosome, using zona-free hamster ova. Our main improvements of methodology are as follows: (1) Fertilization rate of hamster oocytes by human spermatozoa was markedly raised by successive treatments of the spermatozoa with 5-15 microM ionophore A23187 solutions and a capacitation medium (BWW medium) containing 3.5% HSA. The HSA most effective in inducing capacitation was selected from several kinds of HSA products commercially available. (2) Monospermic fertilization was ensured by inseminating oocytes with highly capacitated spermatozoa at a low concentration for a short time. (3) TC medium 199 was used for postinsemination culture of the eggs. (4) A medium containing podophyllotoxin and vinblastine (0.04 micrograms/ml each) was used to block karyogamy and first-cleavage spindle formation. (5) Chromosome slides were prepared with our gradual fixation-air-dry method instead of Tarkowski's method. Ninety-two to 177 spermatozoa corresponding in number to 43%-79% (mean: 62%) of the inseminated oocytes were successfully karyotyped in each experiment. In spite of above-mentioned quantitative improvements, quality of Q-banding was not necessarily satisfactory in our slides. Improvement of banding technique is an important problem to be solved in our method. Spontaneous incidence of chromosome aberrations was studied in a total of 1,091 spermatozoa obtained from nine semen samples from four donors. Incidences of aneuploidy and structural anomaly were 0.9% (hyperhaploidy, 0.45%; hypohaploidy, 0.45%) and 13.0%, respectively. Structural aberrations included breaks (45.1%), fragments (32.4%), exchanges (21.8%), and deletions (0.7%). Ratio of X-sperm to Y-sperm was 53% to 47%. These results were discussed in comparison with those reported previously.
机译:我们已经开发了一种改进的方法,可以使用无透明带的仓鼠卵来分析人的精子染色体。我们对方法的主要改进如下:(1)通过连续用5-15 microM离子载体A23187溶液和含有3.5%HSA的获能培养基(BWW培养基)处理精子,可显着提高人精子对仓鼠卵母细胞的受精率。诱导获能最有效的HSA选自几种市售的HSA产品。 (2)通过在短时间内用低浓度的高获能精子授精卵母细胞来确保单精子受精。 (3)将TC培养基199用于卵的授精后培养。 (4)使用含有鬼臼毒素和长春碱(各自为0.04微克/毫升)的培养基阻止核分裂和第一个分裂纺锤体的形成。 (5)用我们的逐步固定-风干法代替Tarkowski法制备染色体玻片。在每个实验中成功完成了92到177个精子的核型分型,相当于数量的43%-79%(平均:62%)。尽管进行了上述定量改进,但我们的幻灯片中Q带的质量未必令人满意。捆扎技术的改进是我们方法中要解决的重要问题。从四个捐赠者的九个精液样本中获得了总共1,091个精子,研究了染色体畸变的自发发生率。非整倍性和结构异常的发生率分别为0.9%(超单倍体,0.45%;次单倍体,0.45%)和13.0%。结构性畸变包括断裂(45.1%),碎片(32.4%),交换(21.8%)和缺失(0.7%)。 X-精子与Y-精子的比率为53%至47%。将这些结果与先前报告的结果进行了讨论。

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