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Rapid assembly of multiple DNA fragments through direct transformation of PCR products into E.coli and Lactobacillus.

Plasmid.. 2014-09;  76C:40-46
P Cao, L Wang, G Zhou, Y Wang, Y Chen. College of Animal Science and Technology, Northwest A&F University, Yangling 712100, China.
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摘要

This article describes a rapid, highly efficient and versatile method for seamlessly assembling multiple DNA fragments into a vector at any desired position. The inserted fragments and vector backbone were amplified by high-fidelity PCR containing 20 bp to 50 bp overlapping regions at 3' and/or 5' termini. These linearised fragments were equimolarly mixed, and then cyclised in a prolonged overlap extension PCR without adding primers. The resulting PCR products were DNA multimers that could be directly transformed into host strains, yielding the desired chimeric plasmid. The proposed method was illustrated by constructing an Escherichia coli co-expression vector. The feasibility of the method in Lactob... More

关键词

Multiple fragment assembly; Prolong overlap extension PCR; Seamless cloning