Basidiomycete DyPs: Genomic diversity, structural-functional aspects, reaction mechanism and environmental significance

Dolores Linde; Francisco J Ruiz-Dueñas; Elena Fernández-Fueyo; Victor Guallar; Kenneth E Hammel; Rebecca Pogni; Angel T Martínez

doi:10.1016/j.abb.2015.01.018

Basidiomycete DyPs: Genomic diversity, structural-functional aspects, reaction mechanism and environmental significance

Arch Biochem Biophys. 2015 May 15:574:66-74. doi: 10.1016/j.abb.2015.01.018. Epub 2015 Jan 28.

Authors

Dolores Linde¹, Francisco J Ruiz-Dueñas¹, Elena Fernández-Fueyo¹, Victor Guallar², Kenneth E Hammel³, Rebecca Pogni⁴, Angel T Martínez⁵

Affiliations

¹ Centro de Investigaciones Biológicas, CSIC, Ramiro de Maeztu 9, E-28040 Madrid, Spain.
² Joint BSC-CRG-IRB Research Program in Computational Biology, Barcelona Supercomputing Center, Jordi Girona 29, E-08034 Barcelona, Spain; ICREA, Passeig Lluís Companys 23, E-08010 Barcelona, Spain.
³ US Forest Products Laboratory, One Gifford Pinchot Drive, Madison, WI 53726, USA.
⁴ Dept. Biotechnologies, Chemistry and Pharmacy, University of Siena, I-53100 Siena, Italy.
⁵ Centro de Investigaciones Biológicas, CSIC, Ramiro de Maeztu 9, E-28040 Madrid, Spain. Electronic address: ATMartinez@cib.csic.es.

PMID: 25637654
DOI: 10.1016/j.abb.2015.01.018

Abstract

The first enzyme with dye-decolorizing peroxidase (DyP) activity was described in 1999 from an arthroconidial culture of the fungus Bjerkandera adusta. However, the first DyP sequence had been deposited three years before, as a peroxidase gene from a culture of an unidentified fungus of the family Polyporaceae (probably Irpex lacteus). Since the first description, fewer than ten basidiomycete DyPs have been purified and characterized, but a large number of sequences are available from genomes. DyPs share a general fold and heme location with chlorite dismutases and other DyP-type related proteins (such as Escherichia coli EfeB), forming the CDE superfamily. Taking into account the lack of an evolutionary relationship with the catalase-peroxidase superfamily, the observed heme pocket similarities must be considered as a convergent type of evolution to provide similar reactivity to the enzyme cofactor. Studies on the Auricularia auricula-judae DyP showed that high-turnover oxidation of anthraquinone type and other DyP substrates occurs via long-range electron transfer from an exposed tryptophan (Trp377, conserved in most basidiomycete DyPs), whose catalytic radical was identified in the H2O2-activated enzyme. The existence of accessory oxidation sites in DyP is suggested by the residual activity observed after site-directed mutagenesis of the above tryptophan. DyP degradation of substituted anthraquinone dyes (such as Reactive Blue 5) most probably proceeds via typical one-electron peroxidase oxidations and product breakdown without a DyP-catalyzed hydrolase reaction. Although various DyPs are able to break down phenolic lignin model dimers, and basidiomycete DyPs also present marginal activity on nonphenolic dimers, a significant contribution to lignin degradation is unlikely because of the low activity on high redox-potential substrates.

Keywords: CDE superfamily; Catalytic tryptophan; Dye-decolorizing peroxidases; Ligninolysis; Long-range electron transfer; Molecular structure; Reaction mechanism; Substituted anthraquinone breakdown.

Publication types

Research Support, Non-U.S. Gov't
Review

MeSH terms

Basidiomycota / enzymology*
Basidiomycota / genetics
Catalytic Domain
Color
Coloring Agents / metabolism
Genome, Fungal*
Peroxidases / chemistry
Peroxidases / genetics
Peroxidases / metabolism*
Phylogeny
Protein Conformation
Protein Folding

Substances

Coloring Agents
Peroxidases