Mapping and cloning of the par-region of broad-host-range plasmid RP4

Abstract

Various deletion mutants of the identical broad-host-range plasmids RP4 and RK2, obtained after conjugative transfer of these plasmids from Escherichia coli to Alcaligenes eutrophus H16, were tested with respect to their segregation behaviour. Although the parent plasmids and some of the deletion mutants were completely stable in both A. eutrophus and E. coli, other derivatives were lost under non-selective conditions. The analysis of these deletion mutants allowed the identification and mapping of a region encoding a partitioning system ( par) between the tra2 region and the kanamycin resistance gene of RP4 (RK2). This area corresponds to the PstI-C restriction fragment of RP4 (RK2). Cloning of this fragment into several unstable vector plasmids including pBR322 and pACYC177 resulted in all cases in an increase of segregational stability. By insertion of the par-region into an unstable broad-host-range mobilizable plasmid and transfer to a series of gram-negative bacteria, it could be shown that the cloned par-region of RP4 is functional in a broad-host-range.