ADP-ribose diphosphatase

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ADP-ribose diphosphatase
ADP-ribose diphosphatase
Identifiers
EC no.	3.6.1.13
CAS no.	9024-83-3
Databases
IntEnz	IntEnz view
BRENDA	BRENDA entry
ExPASy	NiceZyme view
KEGG	KEGG entry
MetaCyc	metabolic pathway
PRIAM	profile
PDB structures	RCSB PDB PDBe PDBsum
Gene Ontology	AmiGO / QuickGO
PMC
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PMC	articles
PubMed	articles
NCBI	proteins

ADP-ribose diphosphatase (EC 3.6.1.13) is an enzyme that catalyzes a hydrolysis reaction in which water nucleophilically attacks ADP-ribose to produce AMP and D-ribose 5-phosphate. Enzyme hydrolysis occurs by the breakage of a phosphoanhydride bond and is dependent on Mg²⁺ ions that are held in complex by the enzyme.

The C-terminal domain of ADP-ribose diphosphatase contains the Nudix sequence, a highly conserved amino acid sequence that is found in over 450 putative proteins in about 90 different species. A part of this sequence known as the Nudix fold is the catalytic part of the sequence. It is a structurally conserved loop-helix-loop motif that creates a scaffold for metal binding and pyrophosphatase chemistry in the enzyme.^[1]

ADP-ribose hydrolases in general act as protective agents against excessive intracellular accumulation of ADP-ribose, as high intracellular levels of ADP-ribose can be damaging to the cell. ADP-ribose diphosphatase, in particular, hydrolyzes ADP-ribose into AMP and D-ribose 5-phosphate, both of which are intermediates of central metabolic pathways and therefore are easily reused.^[2]^[3]

Other common names for ADP-ribose diphosphatase include ADP-ribose pyrophosphatase and ADPRase. ADP-ribose is commonly referred to as ADPR.

Structure

ADPRase is a dimer of two identical monomers, each of which contain 209 amino acids. The two monomers are folded into two distinct structural domains and with two equivalent catalytic sites. The C-terminal domain consists of the Nudix sequence mentioned above and the N-terminal domain is primarily involved in dimer stabilization. As noted earlier, the Nudix fold is the catalytic part of the enzyme, but both domains are involved in the active site and they both help with the attachment and coordination of H₂O, Mg²⁺, and the ADP-ribose substrate.^[1]

The adjacent picture shows the active site of ADPRase in complex with AMPCPR and Mg²⁺. AMPCPR is a nonhydrolyzable analog of ADP-ribose, and thus functions as an inhibitor of ADPRase. The picture below reveals the first and second Mg²⁺ ions, which serve to coordinate the attacking water molecule so that it is perfectly in line with the scissile bond (O-P-O bond is 177 degrees) and poised for attack. A glutamate side chain (E162) will deprotonate the water molecule, and then the hydroxide ion will attack nucleophilically. This occurs when the water molecule is 3.0 angstroms away from the phosphorus molecule it is attacking. By using H₂O¹⁸, it has been found that the water molecule attacks the adenosyl phosphate. This evidence is a refutation of a previous study that suggested that hydrolysis of ADP-ribose could proceed by nucleophilic attack at either alpha- or beta- phosphate (Gabelli, et al. 2001). After the water molecule attacks, an intermediate is formed, and then ribose 5-phosphate is kicked off as a leaving group. The third active site Mg²⁺ ion is used to stabilize the negative charge of the phosphate group as it leaves, and is thus situated perfectly between the two phosphates.^[4]

When the substrate is bound, the structure of the enzyme differs in shape. With the substrate bound, Loop L9 moves 10 angstroms from its original position in the free enzyme, which forms a tighter turn and brings E162 to its catalytic position, meaning this enzyme cycles between an open (free enzyme) and a closed (substrate-metal complex) conformation. This is important because it prevents nonspecific hydrolysis of other nucleotides.^[4] ADPRase is highly specific for ADPR, as it has been shown that its K_m for ADPR is lower by at least two orders of magnitude than for other sugar nucleotides.

Mechanism

The hydrolysis of ADPR is catalyzed by E162, which improves the nucleophilicity of the water molecule in the active site by deprotonating it. This water is held perfectly in line with the scissile bond by the first and second magnesium ions. The hydroxide ion then attacks the phosphorus atom on the adenosyl phosphate, creating a trigonal bypyramidal intermediate with a negatively charged oxygen attached to the adenosyl phosphate. The double bond is then reformed, effectively discharging ribose 5-phosphate as a leaving group. The third Mg²⁺ is used to stabilize the negative charge on the leaving group.^[4]

Enzyme functions

ADP-ribose is an intermediate that is produced during the metabolism of NAD+, mono- or poly-unsaturated proteins, and cyclic-ADP ribose. ADP-ribose is a protein-glycating agent, and excess levels of ADP-ribose in the cell can cause non-enzymatic ADP-ribosylation. Non-enzymatic ADP-ribosylation can inactivate protein targets that contain nucleotide-binding sites when the adenylate moiety of ADP-ribose binds to them, and it can also interfere with metabolic regulation that occurs via enzymatic ADP-ribosylation.^[3] For example, actin polymerization is inhibited by non-enzymatic ADP-ribosylation at a Cys residue. Thus, it is believed that ADPRase functions in general as a house-cleaning enzyme to eliminate potentially deleterious ADP-ribose from the cell.^[2]^[5]

In the literature, the detoxifying role of ADPRase is directly supported in E. coli cells. But in mammalian cells, there is only an indirect evidence linking ADPRase to a detoxifying role, and this comes from studies of the very specific rat liver ADPRibase-I by cytotoxic agents.^[3]^[6]

References

^ ^a ^b Gabelli SB, Bianchet MA, Bessman MJ, Amzel LM (May 2001). "The structure of ADP-ribose pyrophosphatase reveals the structural basis for the versatility of the Nudix family". Nature Structural Biology. 8 (5): 467–72. doi:10.1038/87647. PMID 11323725. S2CID 10896410.
^ ^a ^b Galperin MY, Moroz OV, Wilson KS, Murzin AG (January 2006). "House cleaning, a part of good housekeeping". Molecular Microbiology. 59 (1): 5–19. doi:10.1111/j.1365-2958.2005.04950.x. PMID 16359314. S2CID 10313196.
^ ^a ^b ^c Ribeiro JM, Carloto A, Costas MJ, Cameselle JC (April 2001). "Human placenta hydrolases active on free ADP-ribose: an ADP-sugar pyrophosphatase and a specific ADP-ribose pyrophosphatase". Biochimica et Biophysica Acta (BBA) - General Subjects. 1526 (1): 86–94. doi:10.1016/S0304-4165(01)00113-1. PMID 11287126.
^ ^a ^b ^c Gabelli SB, Bianchet MA, Ohnishi Y, Ichikawa Y, Bessman MJ, Amzel LM (July 2002). "Mechanism of the Escherichia coli ADP-ribose pyrophosphatase, a Nudix hydrolase". Biochemistry. 41 (30): 9279–85. doi:10.1021/bi0259296. PMID 12135348.
^ Okuda K, Hayashi H, Nishiyama Y (July 2005). "Systematic characterization of the ADP-ribose pyrophosphatase family in the Cyanobacterium Synechocystis sp. strain PCC 6803". Journal of Bacteriology. 187 (14): 4984–91. doi:10.1128/JB.187.14.4984-4991.2005. PMC 1169527. PMID 15995214.
^ Dunn CA, O'Handley SF, Frick DN, Bessman MJ (November 1999). "Studies on the ADP-ribose pyrophosphatase subfamily of the nudix hydrolases and tentative identification of trgB, a gene associated with tellurite resistance". The Journal of Biological Chemistry. 274 (45): 32318–24. doi:10.1074/jbc.274.45.32318. PMID 10542272.

[Gabelliet.al.2001-1] Gabelli SB, Bianchet MA, Bessman MJ, Amzel LM (May 2001). "The structure of ADP-ribose pyrophosphatase reveals the structural basis for the versatility of the Nudix family". Nature Structural Biology. 8 (5): 467–72. doi:10.1038/87647. PMID 11323725. S2CID 10896410.

[Galperinet.al.2006-2] Galperin MY, Moroz OV, Wilson KS, Murzin AG (January 2006). "House cleaning, a part of good housekeeping". Molecular Microbiology. 59 (1): 5–19. doi:10.1111/j.1365-2958.2005.04950.x. PMID 16359314. S2CID 10313196.

[Ribeiroet.al.2001-3] Ribeiro JM, Carloto A, Costas MJ, Cameselle JC (April 2001). "Human placenta hydrolases active on free ADP-ribose: an ADP-sugar pyrophosphatase and a specific ADP-ribose pyrophosphatase". Biochimica et Biophysica Acta (BBA) - General Subjects. 1526 (1): 86–94. doi:10.1016/S0304-4165(01)00113-1. PMID 11287126.

[Gabelliet.al.2002-4] Gabelli SB, Bianchet MA, Ohnishi Y, Ichikawa Y, Bessman MJ, Amzel LM (July 2002). "Mechanism of the Escherichia coli ADP-ribose pyrophosphatase, a Nudix hydrolase". Biochemistry. 41 (30): 9279–85. doi:10.1021/bi0259296. PMID 12135348.

[5] Okuda K, Hayashi H, Nishiyama Y (July 2005). "Systematic characterization of the ADP-ribose pyrophosphatase family in the Cyanobacterium Synechocystis sp. strain PCC 6803". Journal of Bacteriology. 187 (14): 4984–91. doi:10.1128/JB.187.14.4984-4991.2005. PMC 1169527. PMID 15995214.

[pmid10542272-6] Dunn CA, O'Handley SF, Frick DN, Bessman MJ (November 1999). "Studies on the ADP-ribose pyrophosphatase subfamily of the nudix hydrolases and tentative identification of trgB, a gene associated with tellurite resistance". The Journal of Biological Chemistry. 274 (45): 32318–24. doi:10.1074/jbc.274.45.32318. PMID 10542272.

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v t e Enzymes
Activity	Active site Binding site Catalytic triad Oxyanion hole Enzyme promiscuity Diffusion-limited enzyme Cofactor Enzyme catalysis
Regulation	Allosteric regulation Cooperativity Enzyme inhibitor Enzyme activator
Classification	EC number Enzyme superfamily Enzyme family List of enzymes
Kinetics	Enzyme kinetics Eadie–Hofstee diagram Hanes–Woolf plot Lineweaver–Burk plot Michaelis–Menten kinetics
Types	EC1 Oxidoreductases (list) EC2 Transferases (list) EC3 Hydrolases (list) EC4 Lyases (list) EC5 Isomerases (list) EC6 Ligases (list) EC7 Translocases (list)

ADP-ribose diphosphatase

Structure

Mechanism

Enzyme functions

References

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