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Development of Unlabeled Probe Based High‐Resolution Melting Analysis for Detection of Filaggrin Gene Mutation c.3321delA

机译:基于未标记探针的高分辨率熔解分析技术,用于检测丝聚蛋白基因突变c.3321delA

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BackgroundFilaggrin gene (FLG) plays an important role in skin barrier function, and loss-of-function mutations of FLG have been shown to be a predisposing factor for atopic dermatitis (AD). The c.3321delA mutation is the most common FLG mutation in Chinese population. We aim to develop a rapid, cost-efficiency, and reliable closed-tube method that has not been described for the detection of c.3321delA mutation. MethodsRecombinant wild-type and mutant plasmids of c.3321delA mutation were constructed, heterozygous mutant plasmids were prepared by mixing the mutant plasmids and wild-type plasmids at 1:1 ratio. High-resolution melting analysis (HRMA) coupled with an unlabeled DNA probe was employed to identify the shift in melting temperature of the probe–template complex, which reflects the presence of c.3321delA mutation. ResultsUnlabeled probe based HRMA was able to distinguish all three genotypes (wild-type, heterozygote, and mutant) of c.3321delA mutation. Then, we applied this method to genotype 1,317 clinical samples. Genotyping results obtained from unlabeled probe HRMA were 100% concordant with the results from direct sequencing. ConclusionWe developed a fast and high-throughput method to detect the c.3321delA mutation.
机译:背景Filaggrin基因(FLG)在皮肤屏障功能中起着重要作用,并且已证明FLG的功能丧失突变是特应性皮炎(AD)的诱因。 c.3321delA突变是中国人群中最常见的FLG突变。我们的目标是开发一种快速,经济高效且可靠的封闭管方法,该方法尚未描述用于检测c.3321delA突变。方法构建c.3321delA突变的野生型和突变型重组质粒,以1:1的比例混合突变型质粒和野生型质粒,制备杂合型突变型质粒。高分辨率熔解分析(HRMA)与未标记的DNA探针一起用于鉴定探针-模板复合物的解链温度变化,这反映了c.3321delA突变的存在。结果基于未标记探针的HRMA能够区分c.3321delA突变的所有三种基因型(野生型,杂合子和突变体)。然后,我们将该方法应用于基因型1,317个临床样本。从未标记的探针HRMA获得的基因分型结果与直接测序的结果100%一致。结论我们开发了一种快速,高通量的方法来检测c.3321delA突变。

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