A simple two-step, 'hit and fix' method to generate subtle mutations in BACs using short denatured PCR fragments

doi:10.1093/nar/gng080

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Nucleic Acids Research, 2003, Vol. 31, No. 15 e80
© 2003 Oxford University Press

A simple two-step, ‘hit and fix’ method to generate subtle mutations in BACs using short denatured PCR fragments

Yongping Yang and Shyam K. Sharan^*

Mouse Cancer Genetics Program, Center for Cancer Research, National Cancer Institute at Frederick, 1050 Boyles Street, Frederick, MD 21702, USA

*To whom correspondence should be addressed at NCI-Frederick, Building 560/Room 32–31C, PO Box B, Frederick, MD 21702, USA. Tel: +1 301 846 5140; Fax: +1 301 846 6323; Email: ssharan{at}mail.ncifcrf.gov

The bacteriophage lambda recombination system has proven tobe a valuable tool for engineering bacterial artificial chromosomes(BAC). Due to its high efficiency, subtle alterations in theBACs can be generated using oligonucleotides as targeting vectors.Since no selection marker is used, recombinant clones are identifiedutilizing a selective PCR screening method. However, occasionallythe selective PCR screening is not feasible. We describe herea two-step ‘hit and fix’ method that can be reliablyused for generating any subtle alteration in BACs using shortdenatured PCR fragments as targeting vectors. In the first stepof this method, 6–20 nucleotides are changed around thebase where the mutation has to be generated. In the second step,these altered nucleotides are reverted to the original sequenceand simultaneously a subtle alteration is introduced. Sincein each step several nucleotides are changed, PCR primers specificfor such alterations can be designed. This two-step method providesa simple and efficient tool for generating subtle alterationsin BACs that can be very valuable for functional analysis ofgenes.

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