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Specific detection of DNA and RNA targets using a novel isothermal nucleic acid amplification assay based on the formation of a three-way junction structure

机译:DNA和DNA的特异性检测 使用新型等温核酸扩增的RNA靶标 基于三向连接结构形成的分析

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摘要

The formation of DNA three-way junction (3WJ) structures has been utilised to develop a novel isothermal nucleic acid amplification assay (SMART) for the detection of specific DNA or RNA targets. The assay consists of two oligonucleotide probes that hybridise to a specific target sequence and, only then, to each other forming a 3WJ structure. One probe (template for the RNA signal) contains a non-functional single-stranded T7 RNA polymerase promoter sequence. This promoter sequence is made double-stranded (hence functional) by DNA polymerase, allowing T7 RNA polymerase to generate a target-dependent RNA signal which is measured by an enzyme-linked oligosorbent assay (ELOSA). The sequence of the RNA signal is always the same, regardless of the original target sequence. The SMART assay was successfully tested in model systems with several single-stranded synthetic targets, both DNA and RNA. The assay could also detect specific target sequences in both genomic DNA and total RNA from Escherichia coli. It was also possible to generate signal from E.coli samples without prior extraction of nucleic acid, showing that for some targets, sample purification may not be required. The assay is simple to perform and easily adaptable to different targets.
机译:DNA三向连接(3WJ)结构的形成已被用于开发一种新型的等温核酸扩增测定(SMART),用于检测特定的DNA或RNA靶标。该测定法由两个寡核苷酸探针组成,它们与特定的靶序列杂交,然后仅彼此杂交,形成3WJ结构。一种探针(RNA信号的模板)包含无功能的单链T7 RNA聚合酶启动子序列。该启动子序列通过DNA聚合酶制成双链(因此具有功能性),从而允许T7 RNA聚合酶生成靶标依赖性RNA信号,该信号可通过酶联寡吸附测定(ELOSA)进行测量。无论原始靶序列如何,RNA信号的序列始终相同。 SMART分析已在具有多个单链合成靶标(DNA和RNA)的模型系统中成功测试。该测定法还可以检测来自大肠杆菌的基因组DNA和总RNA中的特异性靶序列。也可以从大肠杆菌样品中产生信号而无需事先提取核酸,这表明对于某些靶标, 可能不需要纯化样品。该测定很容易 执行并轻松适应不同目标。

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