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首页> 外文期刊>Folia histochemica et cytobiologica >Modification of equine sperm chromatin decondensation method to use fluorescence in situ hybridization (FISH).
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Modification of equine sperm chromatin decondensation method to use fluorescence in situ hybridization (FISH).

机译:马精子染色质去浓缩方法的改进,以使用荧光原位杂交(FISH)。

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摘要

Fluorescence in situ hybridization (FISH) is widely used in the study of chromosome structure and organization. Cytogenetic evaluation of chromosomes using FISH technique plays an increasingly important role in diagnosing karyotype changes in both somatic and reproductive cells. The aim of the study was to optimize the conditions of stallion sperm decondensation, which have a significant effect on the results of fluorescence in situ hybridization. Appropriate type and time of decondensation was chosen for the sperm of every stallion. It was found that decondensation performed using a preparation incubated in DTT solution for 1.5 minutes and in SDS solution for 10 seconds proved effective for stallions no. 1 and 2. An alternative decondensation method performed in an Eppendorf tube, with incubation in DTT solution for 1 minute and in SDS solution for 5 seconds proved effective for stallions no. 3 and 4. Decondensation using DTT and papain solution, a method successfully used for bull spermatozoa, proved inadequate for horse spermatozoa.
机译:荧光原位杂交(FISH)被广泛用于染色体结构和组织的研究。使用FISH技术对染色体进行细胞遗传学评估在诊断体细胞和生殖细胞的核型变化中起着越来越重要的作用。该研究的目的是优化种马精子的缩合条件,这对荧光原位杂交的结果具有重要影响。为每种种马的精子选择合适的脱凝类型和时间。已经发现,使用在DTT溶液中孵育1.5分钟并在SDS溶液中孵育10秒的制剂进行的缩合被证明对No.2的种有效。 1和2。在Eppendorf管中进行的另一种脱凝方法,在DTT溶液中孵育1分钟,在SDS溶液中孵育5秒证明对No. 1种有效。参见图3和图4。使用DTT和木瓜蛋白酶溶液(一种成功用于牛精子的方法)进行的缩合被证明不足以用于马精子。

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