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Development of a robust and sensitive pyrosequencing assay for the detection of IDH1/2 mutations in gliomas

机译:开发用于检测神经胶质瘤IDH1 / 2突变的可靠而灵敏的焦磷酸测序测定法

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摘要

Assessment of the mutational status of the isocitrate dehydrogenase 1/2 (IDH1/2) gene has become an integral part of the standard diagnostic procedure and, therefore, needs to be accurate. This may, however, be compromised by various factors including the method of analysis and a low tumor cell content. We have developed a rapid, sensitive and robust assay to detect all types of mutation in either IDH1 or IDH2 using pyrosequencing. The efficacy of detecting mutation was evaluated using a panel of control plasmids representing all the different types of IDH1/2 mutation and a set of 160 tumor specimens. The sensitivity of the assays was examined by a serial dilution analysis performed on samples containing various ratios of wild-type and mutant alleles. The pyrosequencing assay detected as little as 5 % of mutant alleles for most mutation types, while conventional Sanger sequencing required the presence of at least 20 % of mutant alleles for identifying mutations. The pyrosequencing assay detected IDH1/2 mutations in three samples which were missed by Sanger sequencing due to their low tumor cell contents. Our assay is particularly useful for the analysis of a large number of specimens as in a retrospective clinical study for example.
机译:异柠檬酸脱氢酶1/2(IDH1 / 2)基因突变状态的评估已成为标准诊断程序的组成部分,因此,需要准确。但是,这可能会受到各种因素的影响,包括分析方法和低肿瘤细胞含量。我们已经开发了一种快速,灵敏且稳定的分析方法,可使用焦磷酸测序来检测IDH1或IDH2中的所有类型的突变。使用代表所有不同类型的IDH1 / 2突变的一组对照质粒和一组160个肿瘤标本评估检测突变的功效。通过对包含各种比例的野生型和突变等位基因的样品进行系列稀释分析,检查了测定的敏感性。对于大多数突变类型,焦磷酸测序检测仅能检测到5%的突变等位基因,而传统的Sanger测序需要至少20%的突变等位基因的存在才能识别突变。焦磷酸测序检测法检测了三个样品中的IDH1 / 2突变,由于它们的肿瘤细胞含量低,Sanger测序遗漏了这些突变。例如,在回顾性临床研究中,我们的测定对于分析大量标本特别有用。

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