An efficient recombination system for chromosome engineering in Escherichia coli

Author:

Yu, D. G.

Ellis, H. M.

Lee, E. C.

Jenkins, N. A.

Copeland, N. G.

Court, D. L.
Author Address

Court DL NCI, Div Basic Sci, Frederick Canc Res & Dev Ctr, Gene Regulat & Chromosome Biol Lab Bldg 539,Room 243 Frederick, MD 21702 USA NCI, Div Basic Sci, Frederick Canc Res & Dev Ctr, Gene Regulat & Chromosome Biol Lab Frederick, MD 21702 USA NCI, Div Basic Sci, Frederick Canc Res & Dev Ctr, Mouse Canc Genet Program Frederick, MD 21702 USA

1. Year: 2000
Journal: Proceedings of the National Academy of Sciences of the United States of America
1. Volume: 97
2. Issue: 11
3. Pages: 5978-5983
Type of Article: Article

Abstract:

A recombination system has been developed for efficient chromosome engineering in Escherichia coil by using electroporated linear DNA. A defective lambda prophage supplies functions that protect and recombine an electroporated linear DNA substrate in the bacterial cell. The use of recombination eliminates the requirement for standard cloning as all novel joints are engineered by chemical synthesis in vitro and the linear DNA is efficiently recombined into place in vivo. The technology and manipulations required are simple and straight forward. A temperature-dependent repressor tightly controls prophage expression, and, thus, recombination functions can be transiently supplied by shifting cultures to 42 degrees C for 15 min. The efficient prophage recombination system does not require host RecA function and depends primarily on Exo, Beta, and Gam functions expressed from the defective lambda prophage, The defective prophage can be moved to other strains and can be easily removed from any strain. Gene disruptions and modifications of both the bacterial chromosome and bacterial plasmids are possible. This system will be especially useful for the engineering of large bacterial plasmids such as those from bacterial artificial chromosome libraries. [References: 37]

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