Expression, Purification, and Characterization of AknX Anthrone Oxygenase, Which Is Involved in Aklavinone Biosynthesis in Streptomyces galilaeus
Anthracenes
0301 basic medicine
Naphthacenes
Molecular Sequence Data
Methyltransferases
Sequence Analysis, DNA
Streptomyces
03 medical and health sciences
Bacterial Proteins
Genes, Bacterial
Multigene Family
Escherichia coli
Mutagenesis, Site-Directed
Oxygenases
Anthracyclines
Amino Acid Sequence
Phylogeny
DOI:
10.1128/jb.184.22.6115-6122.2002
Publication Date:
2002-10-24T20:07:23Z
AUTHORS (5)
ABSTRACT
ABSTRACT
In streptomycete anthracycline biosynthetic gene clusters, small open reading frames are located just upstream of minimal polyketide synthase genes.
aknX
is such a gene found in the aklavinone-aclacinomycin biosynthetic gene cluster of
Streptomyces galilaeus
. In order to identify its function, the
aknX
gene was expressed in
Escherichia coli
. The cell extract prepared from
E. coli
cells overexpressing AknX protein exhibited anthrone oxygenase activity, which converted emodinanthrone to anthraquinone emodin. This indicates that AknX and related gene products such as DnrG and SnoaB are involved in the formation of aklanonic acid from its anthrone precursor, as suggested by their homology with TcmH and ActVA6. The AknX protein fused with a His
6
tag was efficiently purified to homogeneity by Ni
2+
affinity and anion-exchange column chromatography. The native molecular mass of AknX was estimated to be 42 kDa by gel filtration. Thus, native AknX is considered to have a homotrimeric subunit structure. AknX, like TcmH and ActVA6, possesses no apparent prosthetic group for oxygen activation. Site-directed mutagenesis was carried out to identify the key amino acid residue(s) involved in the oxygenation reaction. Of seven AknX mutants expressed, the W67F mutant showed significantly reduced oxygenase activity, suggesting the important role of the W67 residue in the AknX reaction. A possible mechanism for the reaction via peroxy anion intermediate is proposed.
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