Activation of biosynthesis of guanyl-specific ribonuclease secreted by Bacillus circulans under salt stress

The gene transcription of guanyl-specific ribonucleases (RNases), which provide available phosphate to cells of Bacillus, is controlled by the signal transduction system PhoP‒PhoR. However, the biosynthesis of B. circulans RNase does not depend on the signal-transduction regulatory proteins of Pho regulon. It has been found that raising the salt molar concentration in culture medium increases the level of extracellular guanyl-specific ribonuclease Bci synthesized by B. circulans. Sequences homologous to the binding sites of the regulatory protein DegU were found in RNase Bci promoter. The functioning of the DegS–DegU signal transduction system is stimulated by a high salt concentration. Using a strain of B. subtilis that is defective in the DegU regulatory protein, we have shown that the DegS–DegU system participates in the regulation of RNase Bci expression under salt stress.