Mini-lambda: a tractable system for chromosome and BAC engineering

The bacteriophage lambda (lambda) recombination system Red has been used for engineering large DNA fragments cloned into P1 and bacterial artificial chromosomes (BAC or PAC) vectors. So far, this recombination system has been utilized by transferring the BAC or PAC clones into bacterial cells that h...

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Bibliographic Details
Published inGene Vol. 315; pp. 63 - 69
Main Authors Court, Donald L, Swaminathan, Srividya, Yu, Daiguan, Wilson, Helen, Baker, Teresa, Bubunenko, Mikail, Sawitzke, James, Sharan, Shyam K
Format Journal Article
LanguageEnglish
Published Netherlands 02.10.2003
Subjects
Bacteriophage lambda - genetics
Base Sequence
BRCA2 gene
Chromosomes, Artificial, Bacterial - genetics
Chromosomes, Artificial, P1 Bacteriophage - genetics
Cloning, Molecular - methods
DNA Mutational Analysis
DNA, Bacterial - chemistry
DNA, Bacterial - genetics
electroporation
Escherichia coli
Escherichia coli - genetics
Escherichia coli - virology
Genetic Vectors - genetics
Phage ^l
Point Mutation
Prophages - genetics
Recombination, Genetic
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Summary:The bacteriophage lambda (lambda) recombination system Red has been used for engineering large DNA fragments cloned into P1 and bacterial artificial chromosomes (BAC or PAC) vectors. So far, this recombination system has been utilized by transferring the BAC or PAC clones into bacterial cells that harbor a defective lambda prophage. Here we describe the generation of a mini-lambda DNA that can provide the Red recombination functions and can be easily introduced by electroporation into any E. coli strain, including the DH10B-carrying BACs or PACs. The mini-lambda DNA integrates into the bacterial chromosome as a defective prophage. In addition, since it retains attachment sites, it can be excised out to cure the cells of the phage DNA. We describe here the use of the mini-lambda recombination system for BAC modification by introducing a selectable marker into the vector sequence of a BAC clone. In addition, using the mini-lambda, we create a single missense mutation in the human BRCA2 gene cloned in a BAC without the use of any selectable marker. The ability to generate recombinants very efficiently demonstrates the usefulness of the mini-lambda as a very simple mobile system for in vivo genome engineering by homologous recombination, a process named recombineering.
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ISSN:0378-1119
DOI:10.1016/S0378-1119(03)00728-5