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首页> 外文期刊>Molecular BioSystems >Development Of A Multiplexed Bead-based Assay For Detection Of Dna Methylation In Cancer-related Genes
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Development Of A Multiplexed Bead-based Assay For Detection Of Dna Methylation In Cancer-related Genes

机译:癌症相关基因DNA甲基化检测的基于多珠的检测方法的开发

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Herein we report a method for, the detection of methylated CpG dinucleotides located within CpG islands in genomic DNA using multiplexed bead-based assays and standard flow cytometry instrumentation. Four CpG "clusters" were identified in the TFPI2 and SPARC CpG islands whose methylation status was highly correlated with the incidence of invasive cervical cancer in our previous studies. Eight probes in total were designed for both the methylated and unmethylated forms of each cluster and attached to different fluorescently-encoded organosilica bead sets. Probe design was investigated by changing either the length of probes whilst keeping the melting temperature constant, or changing the melting temperature and keeping the probe length constant. Asymmetric polymerase chain reaction (PCR) methods designed without methylation-specific primers were used to prepare fluorescently-labelled targets based on bisulfite-converted genomic DNA. After investigating the specificity of the probes in a model system using fluorescently-labelled synthetic oligonucleotides, cancer cell-line DNA was analysed and the constant length probe design facilitated the correct genotyping of all clusters with respect to negative controls.
机译:在这里,我们报告了一种方法,用于使用基于多重磁珠的测定法和标准流式细胞仪检测位于基因组DNA中CpG岛内的甲基化CpG二核苷酸。在我们先前的研究中,在TFPI2和SPARC CpG岛中发现了四个CpG“簇”,它们的甲基化状态与浸润性宫颈癌的发生率高度相关。针对每个簇的甲基化和未甲基化形式,总共设计了八个探针,并连接到不同的荧光编码的有机硅珠子组。通过在保持熔融温度恒定的同时改变探针的长度或改变熔融温度并使探针长度保持恒定的方式来研究探针设计。设计了不使用甲基化特异性引物的不对称聚合酶链反应(PCR)方法,用于基于亚硫酸氢盐转化的基因组DNA制备荧光标记的靶标。在研究使用荧光标记的合成寡核苷酸的模型系统中探针的特异性后,分析了癌细胞系DNA,恒长度探针设计促进了相对于阴性对照的所有簇的正确基因分型。

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