The order of replication of chromosomal markers inPseudomonas aeruginosastrain 1: I. Marker frequency analysis by transduction

Abstract

SUMMARY: The generalized transducing phage F116 has been used to prepare lysates from fast- and slow-growing cultures ofPseudomonas aeruginosastrain 1. These lysates have been used to transduce a number of auxotrophic markers to prototrophy and the ratios of the numbers of transductants obtained with each lysate have been determined. Since the markers are those which have been mapped by conjugation in previous studies it has been possible to compare the ratios obtained for each marker with the relative position of the marker on the chromosome map. If the assumption is made that there is only one circular chromosome inP. aeruginosastrain 1 it is possible to suggest a way in which two apparently unlinked segments might be joined together. It is also possible to suggest that the chromosome replicates sequentially in two directions from a fixed origin.