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Translation toeprinting assays using fluorescently labeled primers and capillary electrophoresis

机译:使用荧光标记的引物和毛细管电泳进行翻译印迹分析

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摘要

The protocol described here is an adapted version of the toeprinting assay in which the oligonucleotide used to prime the reverse transcription step is labeled with a fluorescent dye instead of 32P. By using a fluorescent dye, the results of the assay are obtained within one hour by direct electrophoresis of the samples on an automated sequencing machine. This eliminates the need to cast and run polyacrylamide gels and to wait to expose dried gels. We show that an identical toeprint was found for the chloramphenicol acetyltransferase transcript using this nonradioactive method, which is in agreement with the previously published 32P-labeled method. Furthermore, in addition to being a faster and safer method, a larger region of sequence can be analyzed with one primer in a single experiment.
机译:此处描述的协议是脚印技术的改进版本,其中用于引发逆转录步骤的寡核苷酸用荧光染料代替32P标记。通过使用荧光染料,通过在自动测序仪上对样品进行直接电泳,可在一小时内获得测定结果。这样就无需浇铸和运行聚丙烯酰胺凝胶,也无需等待暴露干燥的凝胶。我们显示,使用这种非放射性方法发现了氯霉素乙酰转移酶转录物的相同脚印,这与先前发表的32P标记方法一致。此外,除了是一种更快,更安全的方法外,还可以在一个实验中用一个引物分析更大的序列区域。

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