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首页> 外文期刊>Electrophoresis: The Official Journal of the International Electrophoresis Society >Identification of CpG methylation of the SNRPN gene by methylation-specific multiplex PCR.
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Identification of CpG methylation of the SNRPN gene by methylation-specific multiplex PCR.

机译:通过甲基化特异性多重PCR鉴定SNRPN基因的CpG甲基化。

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摘要

In this article, we show that methylation-specific multiplex PCR (MS-multiplex PCR) is a sensitive and specific single assay for detecting CpG methylation status as well as copy number aberrations. We used MS-multiplex PCR to simultaneously amplify three sequences: the 3' ends of the SNRPN gene (for unmethylated sequences), the KRITI gene (as internal control), and the promoter of the SNRPN gene containing CpG islands (for methylated sequences) after digestion with a methylation-sensitive restriction enzyme (HhaI). We established this duplex assay for the analysis of 38 individuals with Prader-Willi syndrome, 2 individuals with Angelman syndrome, and 28 unaffected individuals. By comparing the copy number of the three regions, the methylation status and the copy number changes can be easily distinguished by MS-multiplex PCR without the need of bisulfite treatment of the DNA. The data showed that MS-multiplex PCR allows for the estimation of the methylation level by comparing the copy number aberrationsof unknown samples to the standards with a known methylated status. The in-house-designed MS-multiplex PCR protocol is a relatively simple, cost-effective, and highly reproducible approach as a significant strategy in clinical applications for epigenetics in a routine laboratory.
机译:在本文中,我们显示了甲基化特异性多重PCR(MS-multiple PCR)是一种灵敏且特异性的单一检测方法,用于检测CpG甲基化状态以及拷贝数畸变。我们使用MS多重PCR同时扩增三个序列:SNRPN基因的3'末端(用于未甲基化的序列),KRITI基因(作为内部对照)和包含CpG岛的SNRPN基因的启动子(用于甲基化的序列)用甲基化敏感性限制酶(HhaI)消化后。我们建立了这种双重分析方法,用于分析38例Prader-Willi综合征,2例Angelman综合征和28例未受影响的个体。通过比较三个区域的拷贝数,可以通过MS-multiple PCR轻松区分甲基化状态和拷贝数变化,而无需使用亚硫酸氢盐处理DNA。数据显示,通过将未知样品的拷贝数畸变与具有已知甲基化状态的标准品进行比较,MS多重PCR可以估算甲基化水平。内部设计的MS-multiple PCR方案是一种相对简单,经济高效且可重复性高的方法,是常规实验室中表观遗传学临床应用中的重要策略。

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