[No authors listed]
Ï factors endow RNA polymerase with promoter specificity in bacteria. Extra-Cytoplasmic Function (ECF) Ï factors represent the largest and most diverse family of Ï factors. Most ECF Ï factors must be activated in response to an external signal. One mechanism of activation is the stepwise proteolytic destruction of an anti-Ï factor via Regulated Intramembrane Proteolysis (RIP). In most cases, the site-1 protease required to initiate the RIP process directly senses the signal. Here we report a new mechanism in which the anti-Ï factor rather than the site-1 protease is the sensor. We provide evidence suggesting that the anti-Ï factor RsiV is the bacterial receptor for the innate immune defense enzyme, lysozyme. The site-1 cleavage site is similar to the recognition site of signal peptidase and cleavage at this site is required for ÏV activation in Bacillus subtilis. We reconstitute site-1 cleavage in vitro and demonstrate that it requires both signal peptidase and lysozyme. We demonstrate that the anti-Ï factor RsiV directly binds to lysozyme and muramidase activity is not required for ÏV activation. We propose a model in which the binding of lysozyme to RsiV activates RsiV for signal peptidase cleavage at site-1, initiating proteolytic destruction of RsiV and activation of ÏV. This suggests a novel mechanism in which conformational change in a substrate controls the cleavage susceptibility for signal peptidase. Thus, unlike other ECF Ï factors which require regulated intramembrane proteolysis for activation, the sensor for ÏV activation is not the site-1 protease but the anti-Ï factor.
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