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A rapid and efficient one-tube PCR-based mutagenesis technique using Pfu DNA polymerase

机译:使用Pfu DNA聚合酶的快速高效的基于单管PCR的诱变技术

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摘要

A rapid method for efficiently generating site-directed mutations on a clean sequence background is described. This modification of the megaprimer PCR mutagenesis approach can be performed in one tube in less than 4.5 hours, and does not require purification of intermediate products. High fidelity of DNA sequence replication is obtained by employing Pfu DNA polymerase and limiting the total number of amplification cycles to 30. The mutagenesis efficiency of the procedure is high enough to allow rapid, direct identification of mutants by restriction digest or sequencing techniques.
机译:描述了一种在干净的序列背景上有效产生定点突变的快速方法。 megaprimer PCR诱变方法的这种修改可以在不到4.5小时的时间内在一根试管中完成,并且不需要纯化中间产物。通过使用Pfu DNA聚合酶并将扩增循环的总数限制为30个,可以获得高保真的DNA序列复制。该过程的诱变效率足够高,可以通过限制性酶切或测序技术快速,直接地鉴定突变体。

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