| Literature DB >> 18820909 |
Joaquin Sanchis1, Layla Fernández, J Daniel Carballeira, Jullien Drone, Yosephine Gumulya, Horst Höbenreich, Daniel Kahakeaw, Sabrina Kille, Renate Lohmer, Jérôme J-P Peyralans, John Podtetenieff, Shreenath Prasad, Pankaj Soni, Andreas Taglieber, Sheng Wu, Felipe E Zilly, Manfred T Reetz.
Abstract
Saturation mutagenesis constitutes a powerful method in the directed evolution of enzymes. Traditional protocols of whole plasmid amplification such as Stratagene's QuikChange sometimes fail when the templates are difficult to amplify. In order to overcome such restrictions, we have devised a simple two-primer, two-stage polymerase chain reaction (PCR) method which constitutes an improvement over existing protocols. In the first stage of the PCR, both the mutagenic primer and the antiprimer that are not complementary anneal to the template. In the second stage, the amplified sequence is used as a megaprimer. Sites composed of one or more residues can be randomized in a single PCR reaction, irrespective of their location in the gene sequence.The method has been applied to several enzymes successfully, including P450-BM3 from Bacillus megaterium, the lipases from Pseudomonas aeruginosa and Candida antarctica and the epoxide hydrolase from Aspergillus niger. Here, we show that megaprimer size as well as the direction and design of the antiprimer are determining factors in the amplification of the plasmid. Comparison of the results with the performances of previous protocols reveals the efficiency of the improved method.Entities:
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Year: 2008 PMID: 18820909 DOI: 10.1007/s00253-008-1678-9
Source DB: PubMed Journal: Appl Microbiol Biotechnol ISSN: 0175-7598 Impact factor: 4.813