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Rapid and simultaneous detection of vitamin D receptor gene polymorphisms by a single ARMS-PCR assay

机译:通过单个ARMS-PCR分析快速并同时检测维生素D受体基因多态性

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Background: Vitamin D has various roles in many biological actions such as calcium homeostasis, cell proliferation, and cell differentiation to many target tissues. These effects are mediated by the active form of vitamin D, 1,25(OH)2D3, which binds to a cytoplasmic protein called vitamin D receptor (VDR). VDR gene has four common single nucleotide polymorphisms (SNPs) that are defined by the presence of restriction sites for FokI (F/f), TaqI (T/t), BsmI (B/b), and ApaI (A/a). The association of VDR gene polymorphisms with several diseases has been investigated. In most studies, VDR genotyping was performed by polymerase chain reaction (PCR)-restriction fragment length polymorphism (RFLP) assays, which are cumbersome and time consuming, and their results are sometimes difficult to interpret. Objective: We modified previously reported primers for VDR genotyping and set up a single amplification-refractory mutation system (ARMS)-PCR method for simultaneous genotyping of four common VDR polymorphisms. Methods: In this study, 218 DNA samples were analyzed for VDR genetic variants by this ARMS-PCR technique; 136 of them were re-genotyped by PCR-RFLP assays to compare genotyping results. Result: We obtained allelic frequencies of 69 vs. 31 % for F/f, 34 vs. 66 % for B/b, 70 vs. 30 % for T/t, and 52 vs. 48 % for A/a in this sample of the Iranian population. In addition, comparisons of the results of these two methods showed good uniformity in VDR genotypes; although, in some samples, ambiguity in restriction patterns was present. Conclusion: As ARMS-PCR is more rapid, economic, and user friendly than PCR-RFLP, its substitution would be welcomed in disease association and pharmacogenetic studies of VDR variants.
机译:背景:维生素D在许多生物作用中具有多种作用,例如钙稳态,细胞增殖以及向许多目标组织的细胞分化。这些作用由维生素D的活性形式1,25(OH)2D3介导,该活性形式与称为维生素D受体(VDR)的细胞质蛋白结合。 VDR基因具有四个常见的单核苷酸多态性(SNP),它们由FokI(F / f),TaqI(T / t),BsmI(B / b)和ApaI(A / a)限制性位点的存在定义。已经研究了VDR基因多态性与几种疾病的关系。在大多数研究中,VDR基因分型是通过聚合酶链反应(PCR)-限制性片段长度多态性(RFLP)分析进行的,这既麻烦又费时,而且有时难以解释其结果。目的:我们修改了先前报道的用于VDR基因分型的引物,并建立了一个单一的扩增-难治性突变系统(ARMS)-PCR方法,用于同时进行四种常见VDR多态性的基因分型。方法:在这项研究中,采用ARMS-PCR技术分析了218个DNA样品的VDR基因变异。通过PCR-RFLP分析对其中的136种进行了基因分型,以比较基因分型结果。结果:在该样本中,我们获得了等位基因频率,F / f为69 vs. 31%,B / b为34 vs. 66%,T / t为70 vs. 30%,A / a为52 vs. 48%。伊朗人口。此外,对这两种方法的结果进行比较显示,VDR基因型具有良好的一致性。尽管在某些样本中,限制模式存在歧义。结论:由于ARMS-PCR比PCR-RFLP更加快速,经济和用户友好,在疾病关联和VDR变体的药物遗传学研究中,其替代将受到欢迎。

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