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New insights into the QuikChangeTM process guide the use of Phusion DNA polymerase for site-directed mutagenesis
Author(s) -
Yongzhen Xia,
Wenqiao Chu,
Qingsheng Qi,
Luying Xun
Publication year - 2014
Publication title -
nucleic acids research
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 9.008
H-Index - 537
eISSN - 1362-4954
pISSN - 0305-1048
DOI - 10.1093/nar/gku1189
Subject(s) - biology , plasmid , mutagenesis , site directed mutagenesis , dna , homologous recombination , dna polymerase , genetics , polymerase , microbiology and biotechnology , recombinant dna , in vitro recombination , transformation (genetics) , molecular cloning , mutation , mutant , gene , complementary dna
The QuikChange TM site-directed mutagenesis method is popular but imperfect. An improvement by using partially overlapping primers has been reported several times; however, it is incompatible with the proposed mechanism. The QuikChange TM method using complementary primers is proposed to linearly amplify a target plasmid with the products annealing to produce double-stranded DNA molecules with 5′-overhangs. The overhang annealing is supposed to form circular plasmids with staggered breaks, which can be repaired in Escherichia coli after transformation. Here, we demonstrated that the PCR enzyme fills the 5′-overhangs in the early cycles, and the product is then used as the template for exponential amplification. The linear DNA molecules with homologous ends are joined to generate the plasmid with the desired mutations through homologous recombination in E. coli . The correct understanding is important to method improvements, guiding us to use partially overlapping primers and Phusion DNA polymerase for site-directed mutagenesis. Phusion did not amplify a plasmid with complementary primers but used partially overlapping primers to amplify the plasmid, producing linear DNA molecules with homologous ends for site-directed mutagenesis.

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