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A restriction-free method for gene reconstitution using two single-primer PCRs in parallel to generate compatible cohesive ends

19

Citations

19

References

2017

Year

Abstract

Our method provides an alternative cloning method capable of inserting any DNA fragment of up to at least 20 kb into a plasmid, with high efficiency. This new method does not require restriction sites or alterations of the plasmid or the gene of interest, or additional treatments. The simplicity of both primer design and the procedure itself makes the method suitable for high-throughput cloning and structural genomics.

References

YearCitations

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