We developed a simple method (simple cloning) for subcloning DNA fragments into any location of a targeted vector without the need of restriction enzyme, ligase, exonuclease, or recombinase in Escherichia coli. This technology can be applied to common E. coli hosts (e.g., DH5α, JM109, TOP10, BL21(DE3)). The protocol includes three steps: (1) generate DNA insert and linear vector backbone by regular highfidelity PCR, where these two DNA fragments contain 3′ and 5′ overlapping termini; (2) generate DNA multimers based on these two DNA fragments by using prolonged overlap extension-PCR (POE-PCR) without primers added; and (3) transform POE-PCR product to competent Escherichia coli cells directly, yielding the desired plasmid. Simple cloning provides a new cloning method with great simplicity and flexibility. Furthermore, this new method can be modified for the preparation of a large-size mutant library for directed evolution in E. coli. Using this method, it is very easy to generate a mutant library with a size of more than 107 per 50 μL of the POE-PCR product within 1 day.
CITATION STYLE
Zhong, C., You, C., Wei, P., & Zhang, Y. H. P. (2017). Simple cloning by prolonged overlap extension-PCR with application to the preparation of large-size random gene mutagenesis library in Escherichia coli. In Methods in Molecular Biology (Vol. 1472, pp. 49–61). Humana Press Inc. https://doi.org/10.1007/978-1-4939-6343-0_4
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