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FLAG assay as a novel method for real-time signal generation during PCR: application to detection and genotyping of KRAS codon 12 mutations

机译:FLAG测定法作为PCR期间实时信号产生的新方法:应用于KRAS密码子12突变的检测和基因分型

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摘要

Real-time signal generation methods for detection and characterization of low-abundance mutations in genomic DNA are powerful tools for cancer diagnosis and prognosis. Mutations in codon 12 of the oncogene KRAS, for example, are frequently found in several types of human cancers. We have developed a novel real-time PCR technology, FLAG (FLuorescent Amplicon Generation) and adapted it for simultaneously (i) amplifying mutated codon 12 KRAS sequences, (ii) monitoring in real-time the amplification and (iii) genotyping the exact nucleotide alteration. FLAG utilizes the exceptionally thermostable endonuclease PspGI for real-time signal generation by cleavage of quenched fluorophores from the 5-end of the PCR products and, concurrently, for selecting KRAS mutations over wild type. By including peptide-nucleic-acid probes in the reaction, simultaneous genotyping is achieved that circumvents the requirement for sequencing. FLAG enables high-throughput, closed-tube KRAS mutation detection down to 0.1 mutant-to-wild type. The assay was validated on model systems and compared with allele-specific PCR sequencing for screening 27 cancer specimens. Diverse applications of FLAG for real-time PCR or genotyping applications in cancer, virology or infectious diseases are envisioned.
机译:用于检测和表征基因组DNA中低丰度突变的实时信号生成方法,是癌症诊断和预后的有力工具。例如,在几种类型的人类癌症中经常发现癌基因KRAS的12号密码子突变。我们开发了一种新颖的实时PCR技术FLAG(荧光扩增子产生),并将其同时用于(i)扩增突变的12位密码子KRAS序列,(ii)实时监控扩增和(iii)对确切核苷酸进行基因分型改造。 FLAG利用异常稳定的核酸内切酶PspGI通过切割PCR产物5端的淬灭荧光团来实时生成信号,并同时选择了野生型的KRAS突变。通过在反应中包含肽核酸探针,可以实现同时进行基因分型,从而避免了测序的需要。 FLAG可以实现低通量的突变型至野生型高通量封闭式KRAS突变检测。该测定方法在模型系统上进行了验证,并与等位基因特异性PCR测序进行了比较,以筛选27个癌症标本。设想了FLAG在实时PCR中的不同应用或在癌症,病毒学或传染病中的基因分型应用。

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