Exopolyphosphatases PPX1 and PPX2 from Corynebacterium glutamicum

Corynebacterium glutamicum accumulates up to 300 mM of inorganic polyphosphate (PolyP) in the cytosol or in granules. The gene products of cg0488 (ppx1) and cg1115 (ppx2) were shown to be active as exopolyphosphatases (PPX), as overexpression of either gene resulted in higher exopolyphosphatase activities in crude extracts and deletion of either gene with lower activities than those of the wild-type strain. PPX1 and PPX2 from C. glutamicum share only 25% identical amino acids and belong to different protein groups, which are distinct from enterobacterial, archaeal, and yeast exopolyphosphatases. In comparison to that in the wild type, more intracellular PolyP accumulated in the Δppx1 and Δppx2 deletion mutations but less when either ppx1 or ppx2 was overexpressed. When C. glutamicum was shifted from phosphate-rich to phosphate-limiting conditions, a growth advantage of the deletion mutants and a growth disadvantage of the overexpression strains compared to the wild type were observed. Growth experiments, exopolyphosphatase activities, and intracellular PolyP concentrations revealed PPX2 as being a major exopolyphosphatase from C. glutamicum. PPX2^His was purified to homogeneity and shown to be active as a monomer. The enzyme required Mg²⁺ or Mn²⁺ cations but was inhibited by millimolar concentrations of Mg²⁺, Mn²⁺, and Ca²⁺. PPX2 from C. glutamicum was active with short-chain polyphosphates, even accepting pyrophosphate, and was inhibited by nucleoside triphosphates.Inorganic polyphosphate (PolyP), a linear polymer made of up to hundreds of orthophosphate residues (P_i), has been found in all organisms tested for its presence (3, 4, 7, 12, 20, 22, 48). In nature''s phosphorus cycle, diatom-derived PolyP has recently been shown to be critically important for marine phosphorus sequestration (6). In cells, PolyP may function as a means of storage of phosphorus and/or energy, may substitute ATP in kinase reactions, and was shown to be important in response to many stresses. Mutants of Escherichia coli, Pseudomonas aeruginosa, Shigella spp., Salmonella spp., Vibrio cholerae, and Helicobacter pylori with a low PolyP content showed defects in environmental stress responses and/or virulence (2, 14, 17, 38). In amino acid-starved E. coli, PolyP accumulates and is bound by Lon protease, which degrades ribosomal proteins to liberate amino acids (23).The presence of PolyP granules is used as a diagnostic criterion to distinguish the pathogenic Corynebacterium diphtheriae from nonpathogenic corynebacteria, such as Corynebacterium glutamicum (54). However, these metachromatic granules have recently been shown to be present also in nonpathogenic C. glutamicum (33). When sufficient phosphate is available, C. glutamicum accumulates up to 300 mM of PolyP (24) either soluble in the cytosol or in volutin granules (18, 33). During growth of C. glutamicum on glucose, intracellular PolyP concentrations peaked in the early exponential growth phase and at the entry to stationary phase (18). Soluble PolyP prevailed in the stationary growth phase, while PolyP occurred in granules in the early exponential growth phase (18). C. glutamicum is widely used for the biotechnological production of about 2,200,000 tons of amino acids per year, mainly l-glutamate and l-lysine (50, 58), while the related Corynebacterium ammoniagenes is used for the production of the flavor-enhancing purine nucleotides IMP and XMP (30). As it is conceivable that engineering corynebacterial PolyP metabolism affects overproduction of amino acids or of the phosphorus-containing compounds IMP and XMP, the study of PolyP metabolism and the enzymes involved has recently received increasing attention.PolyP formation in C. glutamicum was shown to be stimulated by MgCl₂ (33), probably due to the magnesium dependence of PolyP synthesizing enzymes (27). In microorganisms, PolyP may be synthesized by PolyP kinases belonging to three distinct families (PPK1, PPK2, and PPK3; EC 2.7.4.1) from ATP or other nucleoside triphosphates (NTPs) in a reversible reaction (12). C. glutamicum possesses two PPK2 genes (ppk2A and ppk2B) (27). Purified PPK2B of C. glutamicum is active as a homotetramer and shows higher catalytic efficiency in the PolyP-forming direction than in the reverse direction, forming NTPs from PolyP. The intracellular PolyP content was increased by overexpression of ppk2B and decreased in the absence of PPK2B (27). Besides PPK2B, no other PolyP-dependent enzyme has been characterized in C. glutamicum, although the cg2091 gene product, a putative PolyP-dependent glucokinase (EC 2.7.1.63), was found to be associated with PolyP granules (33).Degradation of PolyP by hydrolysis may be catalyzed by exopolyphosphatases (PPX) (EC 3.6.1.11) and/or endopolyphosphatases (PPN) (EC 3.6.1.10) (1, 49). Exopolyphosphatases hydrolyze PolyP from the chain''s termini, liberating P_i. The C. glutamicum genome contains two genes encoding putative exopolyphosphatases (ppx1-cg0488 and ppx2-cg1115) (15), but their functions have not yet been characterized. The corresponding proteins are distinct from each other as they share only 25% identical amino acids. Both proteins show 25% amino acid identity to E. coli PPX (1), which possesses 200 additional C-terminal amino acids (56). Here, we have analyzed PolyP degradation in C. glutamicum and show that both cg0488 (ppx1) and cg1115 (ppx2) gene products are functional exopolyphosphatases. Growth experiments, determination of exopolyphosphatase activities, and intracellular PolyP concentrations in strains lacking or overexpressing these genes revealed that cg1115 (ppx2) encodes the major exopolyphosphatase of C. glutamicum, which was characterized enzymatically.