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反转录中用于链特异性基因表达分析和监测引物非依赖型 cDNA 合成的技术。

Technique for strand-specific gene-expression analysis and monitoring of primer-independent cDNA synthesis in reverse transcription.

机构信息

Minerva Foundation Institute for Medical Research, Helsinki, Finland.

出版信息

Biotechniques. 2012 Apr;52(4):263-70. doi: 10.2144/0000113842.

Abstract

Primer-independent cDNA synthesis during reverse transcription hinders quantitative analysis of bidirectional mRNA synthesis in eukaryotes as well as in cells infected with RNA viruses. We report a simple RT-PCR-based assay for strand-specific gene-expression analysis. By modifying the cDNA sequence during reverse transcription, the opposite strands of target sequences can be simultaneously detected by postamplification melting curve analysis and primer-initiated transcripts are readily distinguished from nonspecifically primed cDNA. We have utilized this technique to optimize the specificity of reverse transcription on a panel of 15 target genes. Primer-independent reverse transcription occurred for all target sequences when reverse transcription was performed at 42°C and accounted for 11%-57% of the final PCR amplification products. By raising the reaction temperature to 55°C, the specificity of reverse transcription could be increased without significant loss of sensitivity. We have also demonstrated the utility of this technique for analysis of (+) and (-) RNA synthesis of influenza A virus in infected cells. Thus, this technique represents a powerful tool for analysis of bidirectional RNA synthesis.

摘要

在反转录过程中,引物非依赖性 cDNA 合成会阻碍真核生物以及 RNA 病毒感染细胞中双向 mRNA 合成的定量分析。我们报告了一种基于简单 RT-PCR 的用于链特异性基因表达分析的方法。通过在反转录过程中修饰 cDNA 序列,可以通过扩增后熔解曲线分析同时检测靶序列的相反链,并且可以容易地区分引物起始转录物与非特异性引发的 cDNA。我们已经利用该技术优化了针对 15 个靶基因的反转录特异性。当在 42°C 下进行反转录时,所有靶序列都发生了引物非依赖性反转录,并且占最终 PCR 扩增产物的 11%-57%。通过将反应温度升高到 55°C,可以在不显著降低灵敏度的情况下提高反转录的特异性。我们还证明了该技术在分析感染细胞中流感 A 病毒的(+)和(-)RNA 合成中的应用。因此,该技术代表了分析双向 RNA 合成的有力工具。

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