Thomas Choinowski scite author profile

Laccase is a polyphenol oxidase, which belongs to the family of blue multicopper oxidases. These enzymes catalyze the one-electron oxidation of four reducing-substrate molecules concomitant with the four-electron reduction of molecular oxygen to water. Laccases oxidize a broad range of substrates, preferably phenolic compounds. In the presence of mediators, fungal laccases exhibit an enlarged substrate range and are then able to oxidize compounds with a redox potential exceeding their own. Until now, only one crystal structure of a laccase in an inactive, type-2 copper-depleted form has been reported. We present here the first crystal structure of an active laccase containing a full complement of coppers, the complete polypeptide chain together with seven carbohydrate moieties. Despite the presence of all coppers in the new structure, the folds of the two laccases are quite similar. The coordination of the type-3 coppers, however, is distinctly different. The geometry of the trinuclear copper cluster in the Trametes versicolor laccase is similar to that found in the ascorbate oxidase and that of mammalian ceruloplasmin structures, suggesting a common reaction mechanism for the copper oxidation and the O 2 reduction. In contrast to most blue copper proteins, the type-1 copper in the T. versicolor laccase has no axial ligand and is only 3-fold coordinated. Previously, a modest elevation of the redox potential was attributed to the lack of an axial ligand. Based on the present structural data and sequence comparisons, a mechanism is presented to explain how laccases could tune their redox potential by as much as 200 mV.

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Versatile Peroxidase Oxidation of High Redox Potential Aromatic Compounds: Site-directed Mutagenesis, Spectroscopic and Crystallographic Investigation of Three Long-range Electron Transfer Pathways

Pérez-Boada¹,

Ruíz-Dueñas²,

Pogni³

et al. 2005

Journal of Molecular Biology

240

205

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A Tryptophan Neutral Radical in the Oxidized State of Versatile Peroxidase from Pleurotus eryngii

Pogni

Baratto

Teutloff³

et al. 2006

Journal of Biological Chemistry

117

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Versatile peroxidases are heme enzymes that combine catalytic properties of lignin peroxidases and manganese peroxidases, being able to oxidize Mn 2؉ as well as phenolic and non-phenolic aromatic compounds in the absence of mediators. The catalytic process (initiated by hydrogen peroxide) is the same as in classical peroxidases, with the involvement of 2 oxidizing equivalents and the formation of the so-called Compound I. This latter state contains an oxoferryl center and an organic cation radical that can be located on either the porphyrin ring or a protein residue. In this study, a radical intermediate in the reaction of versatile peroxidase from the ligninolytic fungus Pleurotus eryngii with H 2 O 2 has been characterized by multifrequency (9.4 and 94 GHz) EPR and assigned to a tryptophan residue. Comparison of experimental data and density functional theory theoretical results strongly suggests the assignment to a tryptophan neutral radical, excluding the assignment to a tryptophan cation radical or a histidine radical. Based on the experimentally determined side chain orientation and comparison with a high resolution crystal structure, the tryptophan neutral radical can be assigned to Trp 164 as the site involved in long-range electron transfer for aromatic substrate oxidation.Different heme peroxidases are considered to be involved in the lignin biodegradation process, a key step for carbon recycling in terrestrial ecosystems. These are lignin peroxidase (LiP) 4 and manganese peroxidase (MnP), first described in Phanerochaete chrysosporium (1-3), and the versatile peroxidase (VP), more recently described in fungi from the genera Pleurotus (4 -6) and Bjerkandera (7,8). VP is characterized by combining catalytic properties of the other two ligninolytic peroxidases, MnP and LiP. This enzyme is able to oxidize Mn 2ϩ to Mn 3ϩ and also exhibits manganese-independent activity toward veratryl alcohol and p-dimethoxybenzene. Furthermore, it oxidizes hydroquinones and substituted phenols that are not efficiently oxidized by LiP or MnP in the absence of veratryl alcohol and Mn 2ϩ , respectively. VP is even able to degrade directly high redox potential dyes, which can be eventually oxidized by LiP only in the presence of veratryl alcohol (9, 10).Two genes encoding VP isoenzymes VPL and VPS1, expressed in liquid-and solid-state fermentation cultures, respectively, have been cloned from Pleurotus eryngii (11,12). The deduced amino acid sequences for both isoenzymes were used to build molecular models by homology modeling, taking advantage of sequence identity to P. chrysosporium LiP and MnP and Coprinopsis cinerea (synonym Coprinus cinereus) peroxidase (13). Very recently, the crystal structure of recombinant P. eryngii VP expressed in Escherichia coli and activated in vitro (14) has been determined at 1.33-Å resolution (Protein Data Bank code 2BOQ).Catalytically, VP would follow the classical heme peroxidase cycle, in which hydrogen peroxide is the final electron acceptor, acting as a 2-electron oxidizing substrate f...

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NMR structure of the sterol carrier protein-2: implications for the biological role 1 1Edited by P. E. Wright

García¹,

Szyperski²,

Dyer

et al. 2000

Journal of Molecular Biology

114

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The crystal structure of lignin peroxidase at 1.70 Å resolution reveals a hydroxy group on the C β of tryptophan 171: A novel radical site formed during the redox cycle 1 1Edited by R. Huber

Choinowski¹,

Blodig²,

Winterhalter³

et al. 1999

Journal of Molecular Biology

186

109

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How methionyl-tRNA synthetase creates its amino acid recognition pocket upon l-methionine binding

Serre¹,

Verdon²,

Choinowski³

et al. 2001

Journal of Molecular Biology

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Manganese Oxidation Site in Pleurotus eryngii Versatile Peroxidase: A Site-Directed Mutagenesis, Kinetic, and Crystallographic Study^,

et al. 2006

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The molecular architecture of versatile peroxidase (VP) includes an exposed tryptophan responsible for aromatic substrate oxidation and a putative Mn2+ oxidation site. The crystal structures (solved up to 1.3 A) of wild-type and recombinant Pleurotus eryngii VP, before and after exposure to Mn2+, showed a variable orientation of the Glu36 and Glu40 side chains that, together with Asp175, contribute to Mn2+ coordination. To evaluate the involvement of these residues, site-directed mutagenesis was performed. The E36A, E40A, and D175A mutations caused a 60-85-fold decrease in Mn2+ affinity and a decrease in the Mn2+ oxidation activity. Transient-state kinetic constants showed that reduction of both compounds I and II was affected (80-325-fold lower k2app and 103-104-fold lower k3app, respectively). The single mutants retained partial Mn2+ oxidation activity, and a triple mutation (E36A/E40A/D175A) was required to completely suppress the activity (<1% kcat). The affinity for Mn2+ also decreased ( approximately 25-fold) with the shorter carboxylate side chain in the E36D and E40D variants, which nevertheless retained 30-50% of the maximal activity, whereas similar mutations caused a 50-100-fold decrease in kcat in the case of the Phanerochaete chrysosporium manganese peroxidase (MnP). Additional mutations showed that introduction of a basic residue near Asp175 did not improve Mn2+ oxidation as found for MnP and ruled out an involvement of the C-terminal tail of the protein in low-efficiency oxidation of Mn2+. The structural and kinetic data obtained highlighted significant differences in the Mn2+ oxidation site of the new versatile enzyme compared to P. chrysosporium MnP.

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Structure of Sterol Carrier Protein 2 at 1.8 Å Resolution Reveals a Hydrophobic Tunnel Suitable for Lipid Binding^,

2000

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Sterol carrier protein 2, also known as nonspecific lipid transfer protein is a ubiquitous, small, basic protein of 13 kDa found in animals. Its primary structure is highly conserved between different species, and it has been implicated in the intracellular transport of lipids and in a wide range of other in vitro functions related to sterol and fatty acid metabolism. Sterol carrier protein 2 deficiency in mice leads to elevated concentrations of phytanic acid in the serum and causes hepatocarcinogenesis. However, its actual physiological role is still unknown. Although sterol carrier protein 2 has been studied extensively in the past 20 years, very little is known concerning its three-dimensional structure. The crystal structure of rabbit sterol carrier protein 2, determined at 1.8 A resolution with the MIRAS method, shows a unique alpha/beta-fold. The core of this protein forms a five-stranded antiparallel beta-sheet flanked by five helices. A C-terminal segment (residues 114-123), together with part of the beta-sheet and four alpha-helices, form a hydrophobic tunnel providing the environment for apolar ligands such as fatty acids and fatty acyl-coenzyme As. Structurally well-characterized nonspecific lipid transfer proteins from plants have hydrophobic tunnel-like cavities, which were identified as the binding site for fatty acids and related apolar ligands. Despite the fact that plant nonspecific lipid transfer proteins are smaller proteins than sterol carrier protein 2, show no sequence homology to sterol carrier protein 2, and are structurally unrelated, the cavities of these two classes of proteins are very similar with respect to size, shape, and hydrophobicity, suggesting a common functional role.

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