Multiple site directed mutagenesis strategy based on total RNA and RT-PCR method.

Mol Biotechnol

Department of Plant Physiology and Molecular Plant Biology, Eötvös Loránd University, H-1117, Pázmány Péter sétány 1/C, Budapest, Hungary.

Published: November 2007

AI Article Synopsis

  • Site-directed PCR-based mutagenesis is commonly used to create mutations, but existing methods usually require DNA clones, which aren't always available.
  • The article introduces an improved RT-PCR method that allows for the creation of multiple mutations directly from total RNA, focusing on the human beta-actin gene.
  • The study found that by using specific RT-PCR conditions and three mutagenic primers, they produced seven different clones with a mix of single and multiple mutations, optimizing the process for future applications.

Article Abstract

Site-directed PCR-based mutagenesis methods are widely used to generate mutations. All published methods work on DNA clones carrying the target sequence. However, DNA clones are not always available. We have previously published a RT-PCR-based site-directed mutagenesis method starting from total RNA to overcome this problem. In this article, we report an improvement of our previous method to facilitate introduction of multiple mutations into a target sequence. We demonstrate the efficacy and feasibility of this strategy by mutation of the human beta-actin gene. BamHI restriction endonuclease cleavage sites were generated within the gene to assist screening. Using three mutagenic primers in a single RT-PCR reaction, seven different clones were produced carrying three single and four multiple mutations. An investigation of the effect of the cycle number and elongation time of the PCR reactions revealed that both have an influence on the ratio of clones carrying single and multiple mutations. An optimized protocol was established for efficient multiple site-directed mutagenesis.

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Source
http://dx.doi.org/10.1007/s12033-007-0042-0DOI Listing

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