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Literature DB >> 8750200

A highly efficient procedure for site-specific mutagenesis of full-length plasmids using Vent DNA polymerase.

Abstract

Careful titration of Vent polymerase activity allows efficient amplification of full-length plasmids (12 kb). The high processivity and fidelity of this enzyme made oligonucleotide-directed site-specific mutagenesis of plasmids a straight-forward process. Using only two primers, a mutagenic and a complementary, single-base mutants of recombinant plasmids were obtained consistently with > 90% efficiency from a single round of PCR. This procedure also made site-specific deletion, insertion, and several bases mutagenesis facile and efficient.

Entities: Chemical

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Year: 1995 PMID： 8750200 DOI： 10.1101/gr.5.4.404

Source DB: PubMed Journal: Genome Res ISSN： 1088-9051 Impact factor: 9.043

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Cited

49 in total

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