Moonlighting in bacillus subtilis: The small proteins sr1p and sr7p regulate the moonlighting activity of glyceraldehyde 3‐phosphate dehydrogenase a (gapa) and enolase in RNA degradation

Abstract

Moonlighting proteins are proteins with more than one function. During the past 25 years, they have been found to be rather widespread in bacteria. In Bacillus subtilis, moonlighting has been disclosed to occur via DNA, protein or RNA binding or protein phosphorylation. In addition, two metabolic enzymes, enolase and phosphofructokinase, were localized in the degradosome‐like network (DLN) where they were thought to be scaffolding components. The DLN comprises the major endoribonuclease RNase Y, 3′‐5′ exoribonuclease PnpA, endo/5′‐3′ exoribonucleases J1/J2 and helicase CshA. We have ascertained that the metabolic enzyme GapA is an additional component of the DLN. In addition, we identified two small proteins that bind scaffolding components of the degradosome: SR1P encoded by the dual‐function sRNA SR1 binds GapA, promotes the GapA‐ RNase J1 interaction and increases the RNase J1 activity. SR7P encoded by the dual‐function antisense RNA SR7 binds to enolase thereby enhancing the enzymatic activity of enolase bound RNase Y. We discuss the role of small proteins in modulating the activity of two moonlighting proteins.