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Multiplexed gene expression analysis using the invader RNA assay with MALDI-TOF mass spectrometry detection

机译:使用MALDI-TOF质谱检测的入侵者RNA检测进行多重基因表达分析

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摘要

A mass spectrometric approach for measuring gene expression levels has been developed. Ibis technique utilizes a signal amplification system and analysis by matrix-assisted laser desorption/ionization time-of-flight (MALDI-TOF) mass spectrometry. Signal amplification from the targeted RNA employs a recently developed invasive cleavage assay that does not require prior PCR amplification. The assay uses a set of target-specific probes (oligonucleotides), which hybridize to the RNA being measured to create an overlap structure with a single-stranded flap. This flap is enzymatically cleaved and accumulates linearly in a target-specific manner. The products of the reaction, short DNA oligomers, are well suited for quantitative detection by MALDI-TOF mass spectrometry. Multiplexing is achieved by designing the assays so that reaction products for different mRNA targets have discrete masses that can be resolved in a single mass spectrum. Simultaneous analysis of human cytokine in vitro transcripts IL-1beta, TNF-alpha, and IL-6, with GAPDH as a reference standard, was used as a model system to demonstrate this novel method of gene expression analysis. [References: 31]
机译:已经开发了用于测量基因表达水平的质谱方法。 Ibis技术利用信号放大系统并通过基质辅助激光解吸/电离飞行时间(MALDI-TOF)质谱进行分析。来自靶RNA的信号扩增采用了最近开发的侵入性裂解测定法,不需要事先进行PCR扩增。该测定法使用一组靶标特异性探针(寡核苷酸),这些探针与被测RNA杂交以产生具有单链瓣的重叠结构。该瓣片被酶切并以靶标特异性方式线性积累。该反应的产物,短的DNA低聚物,非常适合通过MALDI-TOF质谱法进行定量检测。通过设计检测方法可以实现多路复用,从而使不同mRNA靶标的反应产物具有可在单个质谱图中解析的离散质量。以GAPDH为参考标准,同时分析人细胞因子体外转录本IL-1beta,TNF-alpha和IL-6,作为模型系统来证明这种新的基因表达分析方法。 [参考:31]

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