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A high-throughput method for quantifying transgene expression in transformed plants with real-time PCR analysis

机译:高通量实时荧光定量PCR分析转化植物中转基因表达的方法

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摘要

When analysing plant transformation in plant transgenic lines, determining the level of transgene expression is essential. Northern blot analysis and reverse-transcription polymerase chain reaction (RT-PCR) are currently used for this purpose and enable qualitative and semiquantitative estimation of transgene mRNA levels. We have introduced a real-time PCR method for quantitative determination of transgene expression level in transgenic potato plants containing the gene for coat protein (CP) of potato virus Y strain NTN (PVYNTN) in order to provide a reliable, high-throughput method that could successfully replace the Northern blot analysis. The method has been compared with other available methods for gene expression analysis with respect to accuracy. sensitivity Specificity. and throughput. The effectiveness of the real-time PCR assay was confirmed on transgenic tobacco plants. It proved to be accurate, sensitive, rapid, and sufficiently reproducible for further application in high-throughput molecular characterisation of transgenic lines. In addition. the described assay enables detection of the virus at increased sensitivity and reproducibility and is therefore appropriate for use in routine PVYNTN detection.
机译:在分析植物转基因品系中的植物转化时,确定转基因表达水平至关重要。 Northern blot分析和逆转录聚合酶链反应(RT-PCR)当前用于此目的,并能够对转基因mRNA水平进行定性和半定量估计。为了提供可靠,高通量的方法,我们引入了一种实时PCR方法,该方法用于定量测定包含马铃薯病毒Y株NTN(PVYNTN)外壳蛋白(CP)基因的转基因马铃薯植物中的转基因表达水平。可以成功取代Northern blot分析。就准确性而言,该方法已与其他用于基因表达分析的方法进行了比较。敏感性特异性。和吞吐量。在转基因烟草植物上证实了实时PCR测定的有效性。它被证明是准确,灵敏,快速且可重现的,可进一步用于转基因品系的高通量分子鉴定。此外。所述的测定使得能够以增加的灵敏度和再现性检测病毒,因此适合用于常规PVYNTN检测。

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