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Determination of CAG repeat length in the androgen-receptor gene using frozen serum.

机译:使用冷冻血清测定雄激素受体基因中的CAG重复长度。

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OBJECTIVES: To determine CAG repeat length in exon one of the androgen-receptor gene, using frozen serum as a source of deoxyribonucleic acid (DNA). METHODS: Samples from previously frozen serum samples were prepared for polymerase chain reaction (PCR) by heating thawed serum to 100 degrees C and subsequent centrifugation at 16,000 g. Three microliters of supernatant were added to the PCR in combination with primers flanking the CAG repeat in exon one of the human androgen-receptor gene. After 35 cycles, the PCR amplicons were electrophoresed on an agarose gel, excised, purified, and sequenced. CAG repeat length was directly determined from DNA sequencing gels. RESULTS: Amplified DNA fragments were obtained after PCR from 140 of the 200 specimens examined to date. The DNA amplicon was successfully sequenced in 111 samples derived from 104 individuals. Within this group, the androgen receptor CAG repeat length varied from 11 to 27. The median CAG repeat length was 21; the lower and upper quartiles were 18 or less and 23 or more, respectively. Results were consistent in each case that CAG repeat length was repetitively determined. CONCLUSIONS: The establishment of a methodology to determine androgen-receptor gene CAG repeat length from frozen serum samples opens multiple new opportunities to explore the potential clinical significance of this genetic polymorphism.
机译:目的:使用冷冻血清作为脱氧核糖核酸(DNA)的来源,确定雄激素受体基因之一外显子中的CAG重复长度。方法:通过将融化的血清加热至100℃,然后以16,000 g离心,来制备先前冷冻的血清样品的样品进行聚合酶链反应(PCR)。将三微升上清液与人雄激素受体基因之一的外显子中位于CAG重复序列侧翼的引物一起添加至PCR。 35个循环后,PCR扩增子在琼脂糖凝胶上电泳,切出,纯化并测序。从DNA测序凝胶直接确定CAG重复长度。结果:PCR扩增后的DNA片段是从迄今检查的200个样本中的140个中获得的。 DNA扩增子成功地测序了104个个体的111个样品。在这一组中,雄激素受体CAG重复长度从11到27不等。下四分位数和上四分位数分别为18或以下和23或以上。在每种情况下,重复确定CAG重复长度的结果都是一致的。结论:一种确定冷冻血清样品中雄激素受体基因CAG重复长度的方法的建立为探索这种遗传多态性的潜在临床意义提供了许多新的机会。

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