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A non-radioactive method for inexpensive quantitative RT-PCR.

机译:一种廉价的定量RT-PCR的非放射性方法。

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摘要

We present a novel method for quantitative RT-PCR that involves direct incorporation of digoxigenin-11-dUTP (DIG-dUTP) during amplification of cDNAs, separation of RT-PCR products by agarose gel electrophoresis, Southern transfer to a nylon membrane, and chemiluminescent detection with an anti-DIG antibody. The whole procedure can be done in about a day and has the following advantages: It is highly sensitive, specificity is confirmed by monitoring the size of the RT-PCR product, it is non-radioactive, quantitative, and does not require expensive specialized equipment.
机译:我们提出了一种定量RT-PCR的新方法,该方法涉及在扩增cDNA期间直接引入地高辛配基-11-dUTP(DIG-dUTP),通过琼脂糖凝胶电泳分离RT-PCR产物,Southern转移至尼龙膜和化学发光用抗DIG抗体进行检测。整个过程可以在一天左右的时间内完成,并具有以下优点:高度敏感,通过监测RT-PCR产品的大小可以确认特异性,它是非放射性的,定量的,不需要昂贵的专用设备。

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