Chorismate mutase

chorismate mutase
Identifiers
EC number 5.4.99.5
CAS number 9068-30-8
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 / EGO
chorismate mutase
Chorismate mutase. Rendered from PDB 2CHS.

In enzymology, a chorismate mutase (EC 5.4.99.5) is an enzyme that catalyzes the chemical reaction for the conversion of chorismate to prephenate in the pathway to the production of phenylalanine and tyrosine, also known as the shikimate pathway.

Reaction

Hence, this enzyme has one substrate, chorismate, and one product, prephenate. Chorismate mutase is found at a branch point in the pathway. The enzyme channels the substrate, chorismate to the biosynthesis of tyrosine and phenylalanine and away from tryptophan.[1] Its role in maintaining the balance of these aromatic amino acids in the cell is vital.[2] This is the single known example of a naturally occurring enzyme catalyzing a pericyclic reaction.[2][nb 1] Chorismate mutase(CM) is only found in fungi, bacteria, and higher plants. This protein may use the morpheein model of allosteric regulation.[4]

Protein family

This enzyme belongs to the family of isomerases, specifically those intramolecular transferases transferring other groups. The systematic name of this enzyme class is chorismate pyruvatemutase. This enzyme is also called hydroxyphenylpyruvate synthase. This enzyme participates in phenylalanine, tyrosine and tryptophan biosynthesis. The structures of chorismate mutase vary in different organisms, but the majority belongs to the AroQ family. The chorismate mutase of this family look most like that of Escherichia coli. That is, they are characterized by an intertwined homodimer of 3-helical subunits. For example, the secondary structure of the CM of yeast is very similar to that of E. coli. Chorimate mutase in the AroQ family are more common in nature and are widely distributed among the prokaryotes.[1] For optimal function, they usually have to be accompanied by another enzyme such as prephanate dehydrogenase.[1] These CM are usually bifunctional enzymes meaning they contain two catalytic capacities in the same polypeptide chain.[1] The CM of eukaryotic organisms are usually monofunctional and are controlled by the aromatic amino acids. There are organisms such as Bacillus subtilis whose chorismate mutase have a completely different structure. These enzymes belong to the AroH family and are characterized by a trimeric α/β barrel topology.[5] CM of this class are monofunctional, containing a single catalytic capacity.

E. coli and Yeast chorismate mutase have a limited sequence homology, but their active sites contain similar residues. The active site of the Yeast chorismate mutase contains Arg16, Arg157, Thr242, Glu246, Glu198, Asn194, and Lys168. The E. coli active site contains the same residues with the exception of these noted exchanges: Asp48 for Asn194, Gln88 for Glu248, and Ser84 for Thr242.[6]

Mechanism of catalysis

The mechanism for the transformation of chorismate to prephenate is formally a Claisen rearrangement. This transformation is the first committed step in the pathway to production of the aromatic amino acids: tyrosine and phenylalanine. In the absence of enzyme catalysis this mechanism proceeds as a concerted, but asynchronous step and is an exergonic process.[2] As a result, there is no formal intermediate, but rather a chair-like transition state. The addition of chorismate mutase, increases the rate of the reaction a million fold. There have been extensive studies on the exact mechanism of this reaction, but the rate-determining step has yet to be uncovered. Some questions that remain surrounding the mechanism are how conformational constraint of the flexible substrate, specific hydrogen bonding to the transition state, and electrostatic interactions actually contribute to catalysis. One study using CM from B. subtilis showed evidence that when a cation was aptly placed in the active site, the electrostatic interactions between it and the negatively charged transition state promoted catalysis.[2]

Notes

  1. Dimethylallyltryptophan synthase has been proposed to catalyze a Cope rearrangement, but this has yet to be proven definitively[3]

References

  1. 1 2 3 4 Qamra R, Prakash P, Aruna B, Hasnain SE, Mande SC (June 2006). "The 2.15 A crystal structure of Mycobacterium tuberculosis chorismate mutase reveals an unexpected gene duplication and suggests a role in host-pathogen interactions". Biochemistry. 45 (23): 6997–7005. doi:10.1021/bi0606445. PMID 16752890.
  2. 1 2 3 4 Kast P, Grisostomi C, Chen IA, Li S, Krengel U, Xue Y, Hilvert D (November 2000). "A strategically positioned cation is crucial for efficient catalysis by chorismate mutase". J. Biol. Chem. 275 (47): 36832–8. doi:10.1074/jbc.M006351200. PMID 10960481.
  3. Luk, L. Y. P.; Qian, Q.; Tanner, M. E. (2011). "A Cope Rearrangement in the Reaction Catalyzed by Dimethylallyltryptophan Synthase?". Journal of the American Chemical Society. 133 (32): 12342–12345. doi:10.1021/ja2034969. PMID 21766851.
  4. T. Selwood & E. K. Jaffe (2011). "Dynamic dissociating homo-oligomers and the control of protein function.". Arch. Biochem. Biophys. 519 (2): 131–43. doi:10.1016/j.abb.2011.11.020. PMC 3298769Freely accessible. PMID 22182754.
  5. Babu M (1999). "Annotation of Chorismate Mutase from the Mycobacterium tuberculosis and the Mycobacterium leprae genome" (PDF). Undergraduate Thesis for the Center of Biotechnology.
  6. Guo H, Cui Q, Lipscomb WN, Karplus M (July 2001). "Substrate conformational transitions in the active site of chorismate mutase: their role in the catalytic mechanism". Proc. Natl. Acad. Sci. U.S.A. 98 (16): 9032–7. doi:10.1073/pnas.141230998. PMC 55368Freely accessible. PMID 11481470.
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