Open AccessDonor plasmids for phenotypically neutral chromosomal gene insertions in Enterobacteriaceae
Author(s) -
Emma R Holden,
Gregory Wickham,
Mark A. Webber,
Nicholas M. Thomson,
Eleftheria Trampari
Publication year - 2020
Publication title -
microbiology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.019
H-Index - 179
eISSN - 1465-2080
pISSN - 1350-0872
DOI - 10.1099/mic.0.000994
Subject(s) - recombineering , recombinase , biology , plasmid , genetics , gene , homologous recombination , locus (genetics) , genome , bacteriophage , computational biology , recombination , escherichia coli
Recombineering using bacteriophage lambda Red recombinase (λ-Red) uses homologous recombination to manipulate bacterial genomes and is commonly applied to disrupt genes to elucidate their function. This is often followed by the introduction of a wild-type copy of the gene on a plasmid to complement its function. This is often not, however, at a native copy number and the introduction of a chromosomal version of a gene can be a desirable solution to provide wild-type copy expression levels of an allele in trans . Here, we present a simple methodology based on the λ-Red-based ‘gene doctoring’ technique, where we developed tools used for chromosomal tagging in a conserved locus downstream of glmS and found no impact on a variety of important phenotypes. The tools described provide an easy, quick and inexpensive method of chromosomal modification for the creation of a library of insertion mutants to study gene function.