Structural and functional insights into phosphomannose isomerase: the role of zinc and catalytic residues

Structural and functional insights into phosphomannose isomerase: the role of zinc and catalytic residues

Phosphomannose isomerase (PMI) is a housekeeping enzyme that is found in organisms ranging from bacteria to fungi to mammals and is important for cell‐wall synthesis, viability and signalling. PMI is a zinc‐dependent enzyme that catalyses the reversible isomerization between mannose 6‐phosphate (M6P...

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Veröffentlicht in:Acta crystallographica. Section D, Biological crystallography. Biological crystallography., 2019-05, Vol.75 (5), p.475-487
Hauptverfasser: Bangera, Mamata, Gowda K, Giri, Sagurthi, S. R., Murthy, M. R. N.
Format: Artikel
Sprache:eng
Schlagworte:
Amino Acids - chemistry
Amino Acids - genetics
Amino Acids - metabolism
Antimicrobial agents
Catalysis
catalytic base
Catalytic Domain
Crystal structure
Crystallography, X-Ray
Enzymes
Fructose
Fructosephosphates - metabolism
Fungi
Isomerism
Isomerization
Mannose
Mannose-6-Phosphate Isomerase - chemistry
Mannose-6-Phosphate Isomerase - genetics
Mannose-6-Phosphate Isomerase - metabolism
Mannosephosphates - metabolism
mechanism of isomerization
Metal ions
Models, Molecular
Mutagenesis, Site-Directed
Mutation
phosphomannose isomerase
Prokaryotes
Protein Conformation
Residues
Ring opening
Salmonella
Salmonella typhimurium - enzymology
Site-directed mutagenesis
Structure-function relationships
Substrate Specificity
Substrates
Viability
Virulence
Zinc
Zinc - chemistry
Zinc - metabolism
zinc binding
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Zusammenfassung:Phosphomannose isomerase (PMI) is a housekeeping enzyme that is found in organisms ranging from bacteria to fungi to mammals and is important for cell‐wall synthesis, viability and signalling. PMI is a zinc‐dependent enzyme that catalyses the reversible isomerization between mannose 6‐phosphate (M6P) and fructose 6‐phosphate (F6P), presumably via the formation of a cis‐enediol intermediate. The reaction is hypothesized to involve ring opening of M6P, the transfer of a proton from the C2 atom to the C1 atom and between the O1 and O2 atoms of the substrate, followed by ring closure resulting in the product F6P. Several attempts have been made to decipher the role of zinc ions and various residues in the catalytic function of PMI. However, there is no consensus on the catalytic base and the mechanism of the reaction catalyzed by the enzyme. In the present study, based on the structure of PMI from Salmonella typhimurium, site‐directed mutagenesis targeting residues close to the bound metal ion and activity studies on the mutants, zinc ions were shown to be crucial for substrate binding. These studies also suggest Lys86 as the most probable catalytic base ing the proton in the isomerization reaction. Plausible roles for the highly conserved residues Lys132 and Arg274 could also be discerned based on comparison of the crystal structures of wild‐type and mutant PMIs. PMIs from prokaryotes possess a low sequence identity to the human enzyme, ranging between 30% and 40%. Since PMI is important for the virulence of many pathogenic organisms, the identification of catalytically important residues will facilitate its use as a potential antimicrobial drug target. Phosphomannose isomerase is a zinc‐dependent enzyme involved in reversible isomerization of mannose 6‐phosphate and fructose 6‐phosphate. Based on extensive site‐directed mutagenesis, structural and biochemical studies on phosphomannose isomerase from Salmonella typhimurium, zinc ions were found to be indispensable for substrate binding and the catalytic base was identified as Lys86.
ISSN:2059-7983
0907-4449
2059-7983
1399-0047
DOI:10.1107/S2059798319004169