6C8T
The structure of MppP soaked with the substrate L-Arg
Summary for 6C8T
| Entry DOI | 10.2210/pdb6c8t/pdb |
| Related | 5DJ1 |
| Descriptor | PLP-Dependent L-Arginine Hydroxylase MppP, (E)-N~2~-({3-hydroxy-2-methyl-5-[(phosphonooxy)methyl]pyridin-4-yl}methylidene)-L-arginine, CHLORIDE ION, ... (5 entities in total) |
| Functional Keywords | dimer, l-arg binding complex, oxidase, plp, antibiotic, oxidoreductase |
| Biological source | Streptomyces wadayamensis More |
| Total number of polymer chains | 4 |
| Total formula weight | 167624.55 |
| Authors | Han, L.,Silvaggi, N.R. (deposition date: 2018-01-25, release date: 2018-09-05, Last modification date: 2023-11-15) |
| Primary citation | Han, L.,Vuksanovic, N.,Oehm, S.A.,Fenske, T.G.,Schwabacher, A.W.,Silvaggi, N.R. Streptomyces wadayamensis MppP is a PLP-Dependent Oxidase, Not an Oxygenase. Biochemistry, 57:3252-3264, 2018 Cited by PubMed Abstract: The PLP-dependent l-arginine hydroxylase/deaminase MppP from Streptomyces wadayamensis (SwMppP) is involved in the biosynthesis of l-enduracididine, a nonproteinogenic amino acid found in several nonribosomally produced peptide antibiotics. SwMppP uses only PLP and molecular oxygen to catalyze a 4-electron oxidation of l-arginine to form a mixture of 2-oxo-4(S)-hydroxy-5-guanidinovaleric acid and 2-oxo-5-guanidinovaleric acid. Steady-state kinetics analysis in the presence and absence of catalase shows that one molecule of peroxide is formed for every molecule of dioxygen consumed in the reaction. Moreover, for each molecule of 2-oxo-4(S)-hydroxy-5-guanidinovaleric acid produced, two molecules of dioxygen are consumed, suggesting that both the 4-hydroxy and 2-keto groups are derived from water. This was confirmed by running the reactions using either O or HO and analyzing the products by ESI-MS. Incorporation of O was only observed when the reaction was performed in HO. Crystal structures of SwMppP with l-arginine, 2-oxo-4(S)-hydroxy-5-guanidinovaleric acid, or 2-oxo-5-guanidinovaleric acid bound were determined at resolutions of 2.2, 1.9. and 1.8 Å, respectively. The structural data show that the N-terminal portion of the protein is disordered unless substrate or product is bound in the active site, in which case it forms a well-ordered helix that covers the catalytic center. This observation suggested that the N-terminal helix may have a role in substrate binding and/or catalysis. Our structural and kinetic characterizations of N-terminal variants show that the N-terminus is critical for catalysis. In light of this new information, we have refined our previously proposed mechanism of the SwMppP-catalyzed oxidation of l-arginine. PubMed: 29473729DOI: 10.1021/acs.biochem.8b00130 PDB entries with the same primary citation |
| Experimental method | X-RAY DIFFRACTION (2.2 Å) |
Structure validation
Download full validation report
