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BRED: A Simple and Powerful Tool for Constructing Mutant and Recombinant Bacteriophage Genomes

by Swigoňová, Zuzana , Balachandran, Amrita , Hatfull, Graham F. , Piuri, Mariana , Oldfield, Lauren M. , Marinelli, Laura J. , van Kessel, Julia C.

in Artificial chromosomes / Bacteria / Bacteriophage lambda - genetics / Cloning, Molecular - methods / Deoxyribonucleic acid / DNA / DNA sequencing / Drug resistance / E coli / Electroporation - methods / Gene Deletion / Gene sequencing / Genes / Genetic engineering / Genetic Engineering - methods / Genetic research / Genome, Viral / Genomes / Genomics / Methods / Microbiology / Molecular Biology / Mutagenesis / Mutagenesis - physiology / Mutants / Mutation / Mycobacterium smegmatis / Mycobacterium tuberculosis / Phages / Plasmids / Proteins / Salmonella / Shigella / Transgenes / Tuberculosis / Vaccines / Virology / Yersinia

2008

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BRED: A Simple and Powerful Tool for Constructing Mutant and Recombinant Bacteriophage Genomes

by Swigoňová, Zuzana , Balachandran, Amrita , Hatfull, Graham F. , Piuri, Mariana , Oldfield, Lauren M. , Marinelli, Laura J. , van Kessel, Julia C.

2008

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BRED: A Simple and Powerful Tool for Constructing Mutant and Recombinant Bacteriophage Genomes

by Swigoňová, Zuzana , Balachandran, Amrita , Hatfull, Graham F. , Piuri, Mariana , Oldfield, Lauren M. , Marinelli, Laura J. , van Kessel, Julia C.

2008

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Journal Article

BRED: A Simple and Powerful Tool for Constructing Mutant and Recombinant Bacteriophage Genomes

Swigoňová, Zuzana,

Balachandran, Amrita,

Hatfull, Graham F.,

Piuri, Mariana,

Oldfield, Lauren M.,

Marinelli, Laura J.,

van Kessel, Julia C.

2008

Overview

Advances in DNA sequencing technology have facilitated the determination of hundreds of complete genome sequences both for bacteria and their bacteriophages. Some of these bacteria have well-developed and facile genetic systems for constructing mutants to determine gene function, and recombineering is a particularly effective tool. However, generally applicable methods for constructing defined mutants of bacteriophages are poorly developed, in part because of the inability to use selectable markers such as drug resistance genes during viral lytic growth. Here we describe a method for simple and effective directed mutagenesis of bacteriophage genomes using Bacteriophage Recombineering of Electroporated DNA (BRED), in which a highly efficient recombineering system is utilized directly on electroporated phage DNA; no selection is required and mutants can be readily detected by PCR. We describe the use of BRED to construct unmarked gene deletions, in-frame internal deletions, base substitutions, precise gene replacements, and the addition of gene tags.

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Publisher

Public Library of Science,Public Library of Science (PLoS)

Subject

Artificial chromosomes

/ Bacteria

/ Bacteriophage lambda - genetics

/ Cloning, Molecular - methods

/ Deoxyribonucleic acid

/ DNA

/ DNA sequencing