Investigation of the Substrate Range of CYP199A4: Modification of the Partition between Hydroxylation and Desaturation Activities by Substrate and Protein Engineering

Investigation of the Substrate Range of CYP199A4: Modification of the Partition between Hydroxylation and Desaturation Activities by Substrate and Protein Engineering

The cytochrome P450 enzyme CYP199A4, from Rhodopseudomonas palustris HaA2, can efficiently demethylate 4‐methoxybenzoic acid. It is also capable of oxidising a range of other related substrates. By investigating substrates with different substituents and ring systems we have been able to show that t...

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Veröffentlicht in:Chemistry : a European journal 2012-12, Vol.18 (52), p.16677-16688
Hauptverfasser: Bell, Stephen G., Zhou, Ruimin, Yang, Wen, Tan, Adrian B. H., Gentleman, Alexander S., Wong, Luet-Lok, Zhou, Weihong
Format: Artikel
Sprache:eng
Schlagworte:
Bacterial Proteins - chemistry
Bacterial Proteins - genetics
Bacterial Proteins - metabolism
Benzoates - chemistry
Binding Sites
Biocatalysis
Chemistry
Crystallography, X-Ray
Cytochrome P-450 Enzyme System - chemistry
Cytochrome P-450 Enzyme System - genetics
Cytochrome P-450 Enzyme System - metabolism
cytochromes
desaturation
Enzyme Activation
Escherichia coli - genetics
Hydroxylation
Methylation
Models, Molecular
Protein Conformation
Protein Engineering
Rhodopseudomonas - enzymology
Substrate Specificity
X-ray crystal structure
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Zusammenfassung:The cytochrome P450 enzyme CYP199A4, from Rhodopseudomonas palustris HaA2, can efficiently demethylate 4‐methoxybenzoic acid. It is also capable of oxidising a range of other related substrates. By investigating substrates with different substituents and ring systems we have been able to show that the carboxylate group and the nature of the ring system and the substituent are all important for optimal substrate binding and activity. The structures of the veratric acid, 2‐naphthoic acid and indole‐6‐carboxylic acid substrate‐bound CYP199A4 complexes reveal the substrate binding modes and the side‐chain conformational changes of the active site residues to accommodate these larger substrates. They also provide a rationale for the selectivity of product oxidation. The oxidation of alkyl substituted benzoic acids by CYP199A4 is more complex, with desaturation reactions competing with hydroxylation activity. The structure of 4‐ethylbenzoic acid‐bound CYP199A4 revealed that the substrate is held in a similar position to 4‐methoxybenzoic acid, and that the Cβ CH bonds of the ethyl group are closer to the heme iron than those of the Cα (3.5 vs. 4.8 Å). This observation, when coupled to the relative energies of the reaction intermediates, indicates that the positioning of the alkyl group relative to the heme iron may be critical in determining the amount of desaturation that is observed. By mutating a single residue in the active site of CYP199A4 (Phe185) we were able to convert the enzyme into a 4‐ethylbenzoic acid desaturase. Engineering a P450 desaturase: The substrate range of CYP199A4 from Rhodopseudomonas palustris was investigated. The partition between the hydroxylation and desaturation activities of 4‐ethylbenzoic acid was studied by changing the substrate and by mutation. The activity of CYP199A4 with 4‐ethylbenzoic acid was changed to a desaturase by a single mutation at F185.
ISSN:0947-6539
1521-3765
DOI:10.1002/chem.201202776