Recombinant circle PCR and recombination PCR for site-specific mutagenesis without PCR product purification
- PMID: 1503755
Recombinant circle PCR and recombination PCR for site-specific mutagenesis without PCR product purification
Abstract
Two simple methods for site-specific mutagenesis are described and compared. In each method, the PCR is used in two separate amplifications to mutate the site of interest and to add ends to one PCR product that are homologous to the ends of the other PCR product. In the first method, the two products are combined, denatured and reannealed prior to transformation of E. coli in order to form recombinant circles in vitro, while in the second method, the two linear products are co-transfected directly into E. coli without prior manipulation, resulting in transformation of E. coli with the recombinant of interest by recombination in vivo. Each PCR amplification uses a plasmid template that has been linearized by restriction enzyme digestion outside the region to be amplified. This permits use of unpurified PCR products in these two protocols and generation of the mutant of interest with no other enzymatic manipulation in vitro apart from PCR amplification. In each protocol greater than or equal to 50% of the resulting clones contained the mutation of interest without detected errors.
Similar articles
-
A rapid method for recombination and site-specific mutagenesis by placing homologous ends on DNA using polymerase chain reaction.Biotechniques. 1991 Jan;10(1):62-6. Biotechniques. 1991. PMID: 2003926
-
A rapid method for site-specific mutagenesis and directional subcloning by using the polymerase chain reaction to generate recombinant circles.Biotechniques. 1990 Feb;8(2):178-83. Biotechniques. 1990. PMID: 2180450
-
Site-directed mutagenesis by combination of homologous recombination and DpnI digestion of the plasmid template in Escherichia coli.Anal Biochem. 2008 Feb 15;373(2):389-91. doi: 10.1016/j.ab.2007.10.034. Epub 2007 Oct 30. Anal Biochem. 2008. PMID: 18037368
-
Using PCR for rapid site-specific mutagenesis in large plasmids.Methods Mol Biol. 1996;57:217-27. doi: 10.1385/0-89603-332-5:217. Methods Mol Biol. 1996. PMID: 8850008 Review. No abstract available.
-
Site-directed mutagenesis using a rapid PCR-based method.Methods Mol Biol. 1996;57:239-48. doi: 10.1385/0-89603-332-5:239. Methods Mol Biol. 1996. PMID: 8850010 Review. No abstract available.
Cited by
-
Ultrabithorax protein is necessary but not sufficient for full activation of decapentaplegic expression in the visceral mesoderm.EMBO J. 1995 Feb 1;14(3):520-35. doi: 10.1002/j.1460-2075.1995.tb07028.x. EMBO J. 1995. PMID: 7859741 Free PMC article.
-
Identification and characterization of a gain-of-function RAG-1 mutant.Mol Cell Biol. 2006 Jun;26(12):4712-28. doi: 10.1128/MCB.02487-05. Mol Cell Biol. 2006. PMID: 16738334 Free PMC article.
-
Stable alteration of pre-mRNA splicing patterns by modified U7 small nuclear RNAs.Proc Natl Acad Sci U S A. 1998 Apr 28;95(9):4929-34. doi: 10.1073/pnas.95.9.4929. Proc Natl Acad Sci U S A. 1998. PMID: 9560205 Free PMC article.
-
Generation of Helper Plasmids Encoding Mutant Adeno-associated Virus Type 2 Capsid Proteins with Increased Resistance against Proteasomal Degradation.Iran J Basic Med Sci. 2013 Jul;16(7):813-21. Iran J Basic Med Sci. 2013. PMID: 23997910 Free PMC article.
-
Ligand-binding domain of an α7-nicotinic receptor chimera and its complex with agonist.Nat Neurosci. 2011 Sep 11;14(10):1253-9. doi: 10.1038/nn.2908. Nat Neurosci. 2011. PMID: 21909087 Free PMC article.
Publication types
MeSH terms
Substances
LinkOut - more resources
Other Literature Sources