Molecular characterization of regulatory elements controlling expression of the Bacillus subtilis recA+ gene

The recA gene of Proteus mirubilk (recApm) has been cloned into the Pat1 site of the Bacillus promoter-probe plasmid pPL603. When present on this plasmid, the rectlpm') gene is expressed in B. subtilie under the control of its own transcriptional and translational signals. It is concluded that the h

Plasmid pC194-1, a mutant of pC194, and chimeric derivatives of pC194-1 are segregationally unstable in B. subtilis. Such instability could be enhanced by exposure of pC194-1-carrying cells to methyl methanesulfonate. pC194-1 is distinct from pC194 in the addition of two A:T base pairs within the pr

Rec mutants of Bacillus subtilis have been tested for complementation by the recA gene of Proteus mirabilis (recApm) which was introduced into B. subtilis via the plasmid pHP334. In the recE4 mutant of B. subtilis the plasmid pHP334 restored significantly the defects in RecE functions tested: UV-sen