9T0V image
Deposition Date 2025-10-20
Release Date 2026-06-10
Last Version Date 2026-06-10
Entry Detail
PDB ID:
9T0V
Keywords:
METAL BINDING PROTEIN
Title:
Crystal structure of H416C NikA mutant from Escherichia coli in complex with Fe(III)-EDTA
Biological Source:
Source Organism(s):
Escherichia coli K-12 (Taxon ID: 83333)
Expression System(s):
Escherichia coli bl21(de3)
Method Details:
Experimental Method:
X-RAY DIFFRACTION
Resolution:
2.54 Å
R-Value Free:
0.25
R-Value Work:
0.20
R-Value Observed:
0.20
Space Group:
P 21 21 21
9T0V validation report missing
Macromolecular Entities
Structures with similar UniProt ID
Protein Blast
Polymer Type:polypeptide(L)
Molecule:Nickel-binding periplasmic pr
Gene (Uniprot):nikA
Mutagens:H416C
Chain IDs:A, B
Chain Length:502
Number of Molecules:2
Biological Source:Escherichia coli K-12
UniProt ID:P33590 Pfam ID:PF00496
Ligand Molecules
ACT
CL
EDT
FE
GOL
SO4
Primary Citation
Covalent Insertion of a Mn(Salen) Type Complex in Cross-Linked Protein Crystals: Design of an Enantioselective Artificial Epoxidase.
Chemistry ? e71159 e71159 (2026)
PMID: 42210913 DOI: 10.1002/chem.71159

Abstact

Artificial enzymes represent a promising alternative for performing non-natural reactions in biocatalysis. Here, we illustrate the potential of cross-linked enzyme crystals (CLEC) to achieve enantioselective epoxidation through the generation of an artificial enzyme obtained by direct covalent anchoring of a manganese complex as an artificial active site within a protein. Enantiomeric excess (ee) of up to 90% on cis-beta-methylstyrene was measured when the covalent binding yield was maximized, thanks to the remarkable behavior of the crystals. The structure of the modified enzyme, NikA, is provided. This work adds to the growing body of examples highlighting the advantages of CLEC in oxidation catalysis.

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Primary Citation of related structures
9T0V
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