Abstract
Streptonigrin methylesterase A (StnA) is one of the tailoring enzymes that modify the aminoquinone skeleton in the biosynthesis pathway of Streptomyces species. Although StnA has no significant sequence homology with the reported α/β-fold hydrolases, it shows typical hydrolytic activity in vivo and in vitro. In order to reveal its functional characteristics, the crystal structures of the selenomethionine substituted StnA (SeMet-StnA) and the complex (S185A mutant) with its substrate were resolved to the resolution of 2.71 Å and 2.90 Å, respectively. The overall structure of StnA can be described as an α-helix cap domain on top of a common α/β hydrolase domain. The substrate methyl ester of 10′-demethoxystreptonigrin binds in a hydrophobic pocket that mainly consists of cap domain residues and is close to the catalytic triad Ser185-His349-Asp308. The transition state is stabilized by an oxyanion hole formed by the backbone amides of Ala102 and Leu186. The substrate binding appears to be dominated by interactions with several specific hydrophobic contacts and hydrogen bonds in the cap domain. The molecular dynamics simulation and site-directed mutagenesis confirmed the important roles of the key interacting residues in the cap domain. Structural alignment and phylogenetic tree analysis indicate that StnA represents a new subfamily of lipolytic enzymes with the specific binding pocket located at the cap domain instead of the interface between the two domains.
Highlights
Sequence homology with reported α/β-fold hydrolases, it is proposed to be an α/β-fold hydrolase that hydrolyzes the methyl ester of 4 towards the production of 5 10
To test the hydrolysis activity of Streptonigrin methylesterase A (StnA) in the production of the compound 5 from the compound 4, StnA was optimized towards the sequence, subsequently overexpressed in E. coli BL21 (DE3) and purified to near homogeneity (Fig. 2A)
StnA is an essential enzyme in the Streptonigrin biosynthesis pathway
Summary
Sequence homology with reported α/β-fold hydrolases, it is proposed to be an α/β-fold hydrolase that hydrolyzes the methyl ester of 4 towards the production of 5 10. The α/β-fold hydrolases family of enzymes is one of the largest groups of structurally related enzymes with diverse catalytic functions Members in this family include proteases, lipases, esterases, dehalogenases, peroxidases, epoxide hydrolases, and others[11]. These enzymes share a common α/βhydrolase fold and a catalytic triad Ser-His-Asp with the Ser residue acting as the nucleophile. The structure of StnA has a unique cap domain that contributes most surface area of the binding pocket This is the first reported case with the specific binding pocket located at the cap domain instead of the interface between the cap domain and the α/βhydrolase fold domain
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