Your search keyword '"Polychaeta enzymology"' showing total 184 results

1. Chromatographic purification of the plasmin-like enzyme from clamworm (Perinereis aibuhitensis Grub) and its fibrinolytic activity by metal ions.

Author

Song T, Han X, Jiang T, Pu X, Wei M, Zhu Y, and Wu W

Subjects

Animals, Hydrogen-Ion Concentration, Polychaeta enzymology, Temperature, Molecular Weight, Enzyme Stability, Metals pharmacology, Electrophoresis, Polyacrylamide Gel, Fibrinolytic Agents isolation & purification, Fibrinolytic Agents chemistry, Fibrinolytic Agents pharmacology, Fibrinolytic Agents metabolism, Fibrinolysin metabolism, Fibrinolysin isolation & purification

Abstract

In this study, fibrinolytic protease was isolated and purified from Perinereis aibuhitensis Grub, and the extraction process was optimized. The properties of the enzyme, such as the amino acid composition, thermal stability, optimal temperature, and pH, were investigated. After detoxification, proteins collected from fresh Clamworm (Perinereis aibuhitensis Grub) were concentrated via ammonium sulfate precipitation. The crude protease was purified using gel filtration resin (Sephadex G-100), anion exchange resin (DEAE-Sepharose FF), and hydrophobic resin (Phenyl Sepharose 6FF). The molecular weight of the protease was determined by polyacrylamide gel electrophoresis (SDS-PAGE). The optimum temperature and optimum pH of the protease were determined. The activity of crude protease in the 40-60% salt-out section was the highest, reaching 467.53 U/mg. The optimal process for purifying crude protein involved the application of DEAE-Sepharose FF and Phenyl Sepharose 6FF, which resulted in the isolation of a single protease known as Asp60-D1-P1 with the highest fibrinolytic activity; additionally, the enzyme activity was measured at 3367.76 U/mg. Analysis by Native-PAGE and SDS-PAGE revealed that the molecular weight of Asp60-D1-P1 was 44.5 kDa, which consisted of two subunits with molecular weights of 6.5 and 37.8 kDa, respectively. The optimum temperature for Asp60-D1-P1 was 40°C, and the optimal pH was 8.0., (© 2024 The Author(s). The FASEB Journal published by Wiley Periodicals LLC on behalf of Federation of American Societies for Experimental Biology.)

Published

2024

2. Oxidation of bisphenol A (BPA) and related compounds by the multifunctional catalytic globin dehaloperoxidase.

Author

Yun D, de Serrano V, and Ghiladi RA

Subjects

Oxidoreductases, Hemoglobins chemistry, Peroxidases metabolism, Phenols, Polychaeta enzymology

Abstract

Dehaloperoxidase (DHP) from the marine polychaete Amphitrite ornata is a multifunctional enzyme that possesses peroxidase, peroxygenase, oxidase and oxygenase activities. Herein, we investigated the reactivity of DHP B with bisphenol A (BPA) and related compounds (bisphenol E, bisphenol F, tetrachlorobisphenol A, 2,2'-biphenol, 3,3'-biphenol, 4,4'-biphenol, and 3,3'-dibromo-4,4'-biphenol). As a previously unknown substrate for DHP B, BPA (as a representative substrate) is an endocrine disruptor widely used in polycarbonate and epoxy resins, thus resulting in human exposure. Reactivity studies with these substrates were investigated using high performance liquid chromatography (HPLC), and their corresponding oxidation products were determined by mass spectrometry (GC-MS/ LC-MS). BPA undergoes oxidation in the presence of DHP B and hydrogen peroxide yielding two cleavage products (4-isopropenylphenol and 4-(2-hydroxypropan-2-yl)phenol), and oligomers with varying degrees of oxidation. 18 O-labeling studies confirmed that the O-atom incorporated into the products was derived exclusively from water, consistent with substrate oxidation via a peroxidase-based mechanism. The X-ray crystal structures of DHP bound with bisphenol E (1.48 Å), bisphenol F (1.75 Å), 2,2'-biphenol (1.90 Å) and 3,3'-biphenol (1.30 Å) showed substrate binding sites are in the distal pocket of the heme cofactor, similar to other previously studied DHP substrates. Stopped-flow UV-visible spectroscopy was utilized to investigate the mechanistic details and enzyme oxidation states during substrate turnover, and a reaction mechanism is proposed. The data presented here strongly suggest that DHP B can catalyze the oxidation of bisphenols and biphenols, thus providing evidence of how infaunal invertebrates can contribute to the biotransformation of these marine pollutants., Competing Interests: Declaration of Competing Interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2022 Elsevier Inc. All rights reserved.)

Published

2023

3. Computational Study of the Peroxygenase Mechanism Catalyzed by Hemoglobin Dehaloperoxidase Involved in the Degradation of Chlorophenols.

Author

Zhang S, Li X, Wang Y, Wei J, Zhang X, and Liu Y

Subjects

Animals, Hemoglobins chemistry, Hemoglobins metabolism, Biocatalysis, Models, Molecular, Density Functional Theory, Polychaeta enzymology, Polychaeta chemistry, Quantum Theory, Chlorophenols chemistry, Chlorophenols metabolism, Peroxidases metabolism, Peroxidases chemistry, Mixed Function Oxygenases metabolism, Mixed Function Oxygenases chemistry

Abstract

The biochemical evidence showed that hemoglobin dehaloperoxidase (DHP B) from Amphitrite Ornata is a multifunctional hemoprotein that catalyzes both dehalogenation and hydroxylation of halophenols via the peroxidase and peroxygenase mechanism, respectively, which sets the basis for the degradation of halophenols. In the peroxygenase mechanism, the reaction was previously suggested to be triggered either by the hydrogen atom abstraction by the Fe═O center or by the proton abstraction by His55. To illuminate the peroxygenase mechanism of DHP B at the atomistic level, on the basis of the high-resolution crystal structure, computational models were constructed, and a series of quantum mechanical/molecular mechanical calculations have been performed. According to the calculation results, the pathway (Path a) initiated by the H-abstraction by the Fe═O center is feasible. In another pathway (Path b), His55 can abstract the proton from the hydroxyl group of the substrate (4-Cl- o -cresol) to initiate the reaction; however, its feasibility depends on the prior electron transfer from the substrate to the porphyrin group. The rate-limiting step of Path a is the OH-rebound, which corresponds to an energy barrier of 14.7 kcal/mol at the quartet state. His55 acts as an acid-base catalyst and directly involves in the catalysis. Our mutant study indicates that His55 can be replaced by other titratable residues. These findings may provide useful information for further understanding of the catalytic reaction of DHP B and for the design of enzymes in the degradation of pollutants, in particular, halophenols.

Published

2022

4. A peroxidase coordinating to Zn (II) preventing heme bleaching and resistant to the interference of H 2 O 2 .

Author

Fu Y, Jiang Z, and Feng W

Subjects

Animals, Catalysis, Oxidants chemistry, Polychaeta enzymology, Zinc metabolism, Chlorophenols chemistry, Heme chemistry, Hemoglobins chemistry, Hemoglobins metabolism, Hydrogen Peroxide chemistry, Peroxidases chemistry, Peroxidases metabolism, Zinc chemistry

Abstract

Dehaloperoxidase (DHP) catalyzes detoxifying halophenols. It is a heme-containing enzyme using H 2 O 2 as the oxidant. Heme bleaching from the active site is of great concern. In addition, the interference of DHP by H 2 O 2 leads to the inactivation of the enzyme. To solve these two problems, DHP is coordinated to Zn (II) in PBS buffer to form a biomineralized composite (DHP&Zn-CP). DHP&Zn-CP was characterized by measuring SEM and confocal images, as well as energy dispersive X-ray spectrometry mapping. Fluorescence spectra demonstrated that DHP&Zn-CP can prevent heme bleaching. Two-dimensional FTIR spectra were measured, dynamically providing insight into the structural change of DHP along the coordination process. Raman spectra were performed to analyze the structural change. The optical spectra confirmed that the forming of DHP&Zn-CP had a little effect on the structures of DHP. For the dehalogenation of 2,4,6-trichlorophenol, DHP&Zn-CP can tolerate the presence of H 2 O 2 and is resistant to the interference by H 2 O 2 . The catalytic efficiency of DHP&Zn-CP is much higher than that of free DHP., (© 2020 American Institute of Chemical Engineers.)

Published

2021

5. The development of early pioneer neurons in the annelid Malacoceros fuliginosus.

Author

Kumar S, Tumu SC, Helm C, and Hausen H

Subjects

Animals, Polychaeta enzymology, Neurogenesis, Neurons cytology, Polychaeta cytology

Abstract

Background: Nervous system development is an interplay of many processes: the formation of individual neurons, which depends on whole-body and local patterning processes, and the coordinated growth of neurites and synapse formation. While knowledge of neural patterning in several animal groups is increasing, data on pioneer neurons that create the early axonal scaffold are scarce. Here we studied the first steps of nervous system development in the annelid Malacoceros fuliginosus., Results: We performed a dense expression profiling of a broad set of neural genes. We found that SoxB expression begins at 4 h postfertilization, and shortly later, the neuronal progenitors can be identified at the anterior and the posterior pole by the transient and dynamic expression of proneural genes. At 9 hpf, the first neuronal cells start differentiating, and we provide a detailed description of axonal outgrowth of the pioneer neurons that create the primary neuronal scaffold. Tracing back the clonal origin of the ventral nerve cord pioneer neuron revealed that it is a descendant of the blastomere 2d (2d 221 ), which after 7 cleavages starts expressing Neurogenin, Acheate-Scute and NeuroD., Conclusions: We propose that an anterior and posterior origin of the nervous system is ancestral in annelids. We suggest that closer examination of the first pioneer neurons will be valuable in better understanding of nervous system development in spirally cleaving animals, to determine the potential role of cell-intrinsic properties in neuronal specification and to resolve the evolution of nervous systems.

Published

2020

6. Luciferase gene of a Caribbean fireworm (Syllidae) from Puerto Rico.

Author

Mitani Y, Yasuno R, Futahashi R, Oakley TH, and Ohmiya Y

Subjects

Amino Acid Sequence, Animals, Japan, Luciferases genetics, Polychaeta metabolism, Puerto Rico, Recombinant Proteins genetics, Sequence Homology, Luciferases metabolism, Luminescence, Polychaeta enzymology, Polychaeta genetics, Recombinant Proteins metabolism

Abstract

The fireworms Odontosyllis spp. are globally distributed and well-known for their characteristic and fascinating mating behavior, with secreted mucus emitting bluish-green light. However, knowledge about the molecules involved in the light emission are still scarce. The fireworms are believed to emit light with a luciferin-luciferase reaction, but biochemical evidence of the luciferase is established for only one species living in Japan and no information is available for its luciferin structure. In this study, we identified a luciferase gene from a related Puerto Rican fireworm. We identified eight luciferase-like genes in this Puerto Rican fireworm, finding amino acid identities between Japanese and Puerto Rican luciferase-like genes to be less than 60%. We confirmed cross reactivity of extracts of the Japanese fireworm luciferin with a recombinant Puerto Rican luciferase (PR1). The emission spectrum of recombinant PR1 was similar to the crude extract of the native luciferase, suggesting that PR1 is a functional luciferase of this Puerto Rican fireworm. Our results indicate that the molecular mechanism of luminescence is widely conserved among fireworms.

Published

2019

7. Spatio-temporal variability of biomarker responses and lipid composition of Marphysa sanguinea, Montagu (1813) in the anthropic impacted lagoon of Tunis.

Author

Mdaini Z, El Cafsi M, Tremblay R, Pharand P, and Gagné JP

Subjects

Animals, Antioxidants metabolism, Ecotoxicology, Environmental Biomarkers drug effects, Mediterranean Sea, Metals, Heavy toxicity, Polychaeta enzymology, Polychaeta metabolism, Seasons, Spatio-Temporal Analysis, Trace Elements toxicity, Tunisia, Water Pollutants, Chemical toxicity, Environmental Monitoring methods, Lipids chemistry, Metals, Heavy analysis, Polychaeta drug effects, Trace Elements analysis, Water Pollutants, Chemical analysis

Abstract

In this study the Polychaeta Marphysa sanguinea, was tested to investigate the impact of metal pollution on the environmental state of a coastal Mediterranean lagoon, Tunis Lagoon (Tunisia). A multi-biomarker approach comprising glutathione-stransferase, cyclooxygenase, lysozyme activity, and lipid class composition of the Polychaeta was employed on a seasonal basis in the present investigation. The multivariate statistical approach (principal component analysis and Pearson correlation) clearly demonstrated different spatial patterns in biomarker values and lipid class concentrations. The phospholipids were the dominant lipid class in M. sanguinea, with the highest value found at the control station. The impact of pollution was most clearly observed on the main storage lipid class, triacylglycerol, which was lowest in the most impacted sites. Our work suggests that M. sanguinea can be used in warmer Mediterranean costal habitats as a sentinel species of contaminated ecosystems., (Copyright © 2019 Elsevier Ltd. All rights reserved.)

Published

2019

8. Sub-lethal Responses of the Polychaete Armandia agilis in Whole-sediment Toxicity Testing.

Author

da Silva Toscano Saes RV, Moreira LB, Peres TF, Taniguchi S, Bícego MC, Marins RV, and de Souza Abessa DM

Subjects

Acetylcholinesterase metabolism, Animals, Catalase metabolism, Environmental Monitoring methods, Glutathione Transferase metabolism, Polychaeta enzymology, Toxicity Tests, Geologic Sediments chemistry, Polychaeta drug effects, Water Pollutants, Chemical toxicity

Abstract

The present study assessed biochemical responses as sublethal endpoints in the polychaete Armandia agilis exposed to contaminated sediments to in order to assess its potential use as a test organism. Sediment samples from several locations at a dredging site were obtained and used in whole-sediment exposures. Samples were tested with A. agilis to determine the 10-day toxicity of the 100% sample and the enzymatic activity of catalase (CAT), glutathione-S-transferase (GST) and acetylcholinesterase (AChE) biochemical measurements made in whole-body homogenates of a subset of the surviving organisms. Biochemical responses reported in A. agilis were not statistically different from the reference site sediment, however, the integrated analysis demonstrated that contaminants bound to sediment samples influenced the sublethal effects.

Published

2019

9. Peroxidase versus Peroxygenase Activity: Substrate Substituent Effects as Modulators of Enzyme Function in the Multifunctional Catalytic Globin Dehaloperoxidase.

Author

McGuire AH, Carey LM, de Serrano V, Dali S, and Ghiladi RA

Subjects

Animals, Crystallography, X-Ray, Guaiacol analogs & derivatives, Halogenation, Hemoglobins chemistry, Hydrogen Peroxide metabolism, Models, Molecular, Oxidation-Reduction, Peroxidases chemistry, Polychaeta chemistry, Polychaeta metabolism, Substrate Specificity, Guaiacol metabolism, Hemoglobins metabolism, Peroxidases metabolism, Polychaeta enzymology

Abstract

The dehaloperoxidase-hemoglobin (DHP) from the terebellid polychaete Amphitrite ornata is a multifunctional hemoprotein that catalyzes the oxidation of a wide variety of substrates, including halo/nitrophenols, haloindoles, and pyrroles, via peroxidase and/or peroxygenase mechanisms. To probe whether substrate substituent effects can modulate enzyme activity in DHP, we investigated its reactiviy against a panel of o-guaiacol substrates given their presence (from native/halogenated and non-native/anthropogenic sources) in the benthic environment that A. ornata inhabits. Using biochemical assays supported by spectroscopic, spectrometric, and structural studies, DHP was found to catalyze the H 2 O 2 -dependent oxidative dehalogenation of 4-haloguaiacols (F, Cl, and Br) to 2-methoxybenzoquinone (2-MeOBQ). 18 O labeling studies confirmed that O atom incorporation was derived exclusively from water, consistent with substrate oxidation via a peroxidase-based mechanism. The 2-MeOBQ product further reduced DHP to its oxyferrous state, providing a link between the substrate oxidation and O 2 carrier functions of DHP. Nonnative substrates resulted in polymerization of the initial substrate with varying degrees of oxidation, with 2-MeOBQ identified as a minor product. When viewed alongside the reactivity of previously studied phenolic substrates, the results presented here show that simple substituent effects can serve as functional switches between peroxidase and peroxygenase activities in this multifunctional catalytic globin. More broadly, when recent findings on DHP activity with nitrophenols and azoles are included, the results presented here further demonstrate the breadth of heterocyclic compounds of anthropogenic origin that can potentially disrupt marine hemoglobins or function as environmental stressors, findings that may be important when assessing the environmental impact of these pollutants (and their metabolites) on aquatic systems.

Published

2018

10. Luciferase of the Japanese syllid polychaete Odontosyllis undecimdonta.

Author

Schultz DT, Kotlobay AA, Ziganshin R, Bannikov A, Markina NM, Chepurnyh TV, Shakhova ES, Palkina K, Haddock SHD, Yampolsky IV, and Oba Y

Subjects

Amino Acid Sequence, Animals, Evolution, Molecular, Japan, Luciferases genetics, Luminescence, Polychaeta genetics, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Sequence Homology, Amino Acid, Structural Homology, Protein, Luciferases chemistry, Luciferases metabolism, Polychaeta enzymology

Abstract

Odontosyllis undecimdonta is a marine syllid polychaete that produces bright internal and exuded bioluminescence. Despite over fifty years of biochemical investigation into Odontosyllis bioluminescence, the light-emitting small molecule substrate and catalyzing luciferase protein have remained a mystery. Here we describe the discovery of a bioluminescent protein fraction from O. undecimdonta, the identification of the luciferase using peptide and RNA sequencing, and the in vitro reconstruction of the bioluminescence reaction using highly purified O. undecimdonta luciferin and recombinant luciferase. Lastly, we found no identifiably homologous proteins in publicly available datasets. This suggests that the syllid polychaetes contain an evolutionarily unique luciferase among all characterized luminous taxa., (Copyright © 2018 Elsevier Inc. All rights reserved.)

Published

2018

11. Sabellastarte magnifica Carboxypeptidase Inhibitor: The first Kunitz inhibitor simultaneously interacting with carboxypeptidases and serine proteases.

Author

Reytor González ML, Alonso-Del-Rivero Antigua M, Hedstrom L, Kuzmič P, and Pires JR

Subjects

Animals, Kinetics, Magnetic Resonance Spectroscopy, Trypsin chemistry, Trypsin metabolism, Carboxypeptidases antagonists & inhibitors, Carboxypeptidases metabolism, Polychaeta enzymology, Protease Inhibitors chemistry, Serine Proteases metabolism

Abstract

Multi-domain inhibitors capable to block the activity of different classes of proteases are not very common in nature. However, these kinds of molecules are attractive systems for biomedical or biotechnological applications, where two or more different targets need to be neutralized. SmCI, the Sabellastarte magnifica Carboxypeptidase Inhibitor, is a tri-domain BPTI-Kunitz inhibitor capable to inhibit serine proteases and A-like metallocarboxypeptidases. The BPTI-Kunitz family of proteins includes voltage gated channel blockers and inhibitors of serine proteases. SmCI is therefore, the only BPTI-Kunitz protein capable of inhibiting metallocarboxypeptidases. The X-ray structure of the SmCI-carboxypeptidase A complex previously obtained by us, revealed that this enzyme interacts with SmCI N-tail. In the complex, the reactive loops for serine protease inhibition remain fully exposed to the solvent in each domain, suggesting SmCI can simultaneously interact with multiple serine proteases. The twofold goals of this study were: i) to establish serine proteases-SmCI binding stoichiometry, given that the inhibitor is comprised of three potential binding domains; and ii) to determine whether or not SmCI can simultaneously bind both classes of enzymes, to which it binds individually. Our experimental approach included a variety of techniques for the study of protein-protein interactions, using as model enzymes pancreatic trypsin, elastase and carboxypeptidase A. In particular, we combined information obtained from gel filtration chromatography, denaturing electrophoresis, nuclear magnetic resonance spectroscopy and enzyme inhibition assays. Our results show that SmCI is able to bind three trypsin molecules under saturating conditions, but only one elastase interacts with the inhibitor. Additionally, we demonstrated that SmCI can bind serine proteases and carboxypeptidases at the same time (at least in the ratio 1:1:1), becoming the first protease inhibitor that simultaneously blocks these two mechanistic classes of enzymes., (Copyright © 2018 Elsevier B.V. and Société Française de Biochimie et Biologie Moléculaire (SFBBM). All rights reserved.)

Published

2018

12. Baseline levels of biochemical biomarkers in the endobenthic ragworm Hediste diversicolor as useful tools in biological monitoring of estuaries under anthropogenic pressure.

Author

Barrick A, Marion JM, Perrein-Ettajani H, Châtel A, and Mouneyrac C

Subjects

Animals, Ecosystem, France, Models, Theoretical, Polychaeta drug effects, Salinity, Biomarkers analysis, Environmental Monitoring methods, Estuaries, Polychaeta enzymology, Rivers chemistry, Water Pollutants, Chemical analysis

Abstract

Identification of contamination in estuarine ecosystems that are impacted by anthropogenic pressures, such as the Seine estuary, is difficult to determine without considering the role environmental variation plays on the end points selected. Currently, there is interest in identifying methods in which the influence of confounding factors can be described and accounted for. In this context, the aim of this study was to define a baseline assessment criteria (BAC) for enzymatic biomarkers in ragworms (Hediste diversicolor) collected in a reference site (Authie). The model took into consideration the weight, temperature and salinity of the site. Values collected in the Seine estuary were analyzed with the model to determine if differences between the sites could potentially be due to contamination or were explained by environmental variation. In general, biomarker responses from the Seine estuary fell within the range of BAC, suggesting that environmental variation could explain some of the results., (Copyright © 2018 Elsevier Ltd. All rights reserved.)

Published

2018

13. Dynamics of dehaloperoxidase-hemoglobin A derived from NMR relaxation spectroscopy and molecular dynamics simulation.

Author

Zhao J, Xue M, Gudanis D, Gracz H, Findenegg GH, Gdaniec Z, and Franzen S

Subjects

Algorithms, Animals, Binding Sites, Crystallography, X-Ray, Dimerization, Hemoglobins chemistry, Hemoglobins genetics, Histidine chemistry, Histidine genetics, Histidine metabolism, Kinetics, Ligands, Molecular Dynamics Simulation, Nitrogen Isotopes, Nuclear Magnetic Resonance, Biomolecular, Oligopeptides chemistry, Oligopeptides genetics, Oligopeptides metabolism, Peroxidases chemistry, Peroxidases genetics, Protein Conformation, Protein Folding, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins metabolism, Xenon chemistry, Xenon metabolism, Hemoglobins metabolism, Models, Molecular, Peroxidases metabolism, Polychaeta enzymology

Abstract

Dehaloperoxidase-hemoglobin is the first hemoglobin identified with biologically-relevant oxidative functions, which include peroxidase, peroxygenase and oxidase activities. Herein we report a study of the protein backbone dynamics of DHP using heteronuclear NMR relaxation methods and molecular dynamics (MD) simulations to address the role of protein dynamics in switching from one function to another. The results show that DHP's backbone helical regions and turns have average order parameters of S 2  = 0.87 ± 0.03 and S 2  = 0.76 ± 0.08, respectively. Furthermore, DHP is primarily a monomer in solution based on the overall tumbling correlation time τ m is 9.49 ± 1.65 ns calculated using the prolate diffusion tensor model in the program relax. A number of amino acid residues have significant R ex using the Lipari-Szabo model-free formalism. These include Lys 3 , Ile 6 , Leu 13 , Gln 18 , Arg 32 , Ser 48 , Met 49 , Thr 56 , Phe 60 , Arg 69 , Thr 71 Cys 73 , Ala 77 , Asn 81 , Gly 95 , Arg 109 , Phe 115 , Leu 127 and Met 136 , which may experience slow conformational motions on the microseconds-milliseconds time scale according to the model. Caution should be used when the model contains >4 fitting parameters. The program caver3.0 was used to identify tunnels inside DHP obtained from MD simulation snapshots that are consistent with the importance of the Xe binding site, which is located at the central intersection of the tunnels. These tunnels provide diffusion pathways for small ligands such as O 2 , H 2 O and H 2 O 2 to enter the distal pocket independently of the trajectory of substrates and inhibitors, both of which are aromatic molecules., (Copyright © 2018 Elsevier Inc. All rights reserved.)

Published

2018

14. Selective tuning of activity in a multifunctional enzyme as revealed in the F21W mutant of dehaloperoxidase B from Amphitrite ornata.

Author

Carey LM, Kim KB, McCombs NL, Swartz P, Kim C, and Ghiladi RA

Subjects

Animals, Catalysis, Crystallography, X-Ray, Hemoglobins chemistry, Hemoglobins genetics, Hemoglobins isolation & purification, Peroxidases chemistry, Peroxidases genetics, Peroxidases isolation & purification, Spectrophotometry, Ultraviolet, Substrate Specificity, Hemoglobins metabolism, Mutation, Peroxidases metabolism, Polychaeta enzymology

Abstract

Possessing both peroxidase and peroxygenase activities with a broad substrate profile that includes phenols, indoles, and pyrroles, the enzyme dehaloperoxidase (DHP) from Amphitrite ornata is a multifunctional catalytic hemoglobin that challenges many of the assumptions behind the well-established structure-function paradigm in hemoproteins. While previous studies have demonstrated that the F21W variant leads to attenuated peroxidase activity in DHP, here we have studied the impact of this mutation on peroxygenase activity to determine if it is possible to selectively tune DHP to favor one function over another. Biochemical assays with DHP B (F21W) revealed minimal decreases in peroxygenase activity of 1.2-2.1-fold as measured by 4-nitrophenol or 5-Br-indole substrate conversion, whereas the peroxidase activity catalytic efficiency for 2,4,6-trichlorophenol (TCP) was more than sevenfold decreased. Binding studies showed a 20-fold weaker affinity for 5-bromoindole (K d  = 2960 ± 940 μM) in DHP B (F21W) compared to WT DHP B. Stopped-flow UV/visible studies and isotope labeling experiments together suggest that the F21W mutation neither significantly changes the nature of the catalytic intermediates, nor alters the mechanisms that have been established for peroxidase and peroxygenase activities in DHP. The X-ray crystal structure (1.96 Å; PDB 5VLX) of DHP B (F21W) revealed that the tryptophan blocks one of the two identified TCP binding sites, specifically TCP interior , suggesting that the other site, TCP exterior , remains viable for binding peroxygenase substrates. Taken together, these studies demonstrate that blocking the TCP interior binding site in DHP selectively favors peroxygenase activity at the expense of its peroxidase activity.

Published

2018

15. A Novel Thrombolytic and Anticoagulant Serine Protease from Polychaeta, Diopatra sugokai .

Author

Kim HJ, Shim KH, Yeon SJ, and Shin HS

Subjects

Amino Acid Sequence, Animals, Cell Line drug effects, Cell Survival drug effects, Endothelial Cells drug effects, Enzyme Activation, Enzyme Assays, Fibrinogen metabolism, Hydrogen-Ion Concentration, Temperature, Tissue Plasminogen Activator, Anticoagulants isolation & purification, Anticoagulants metabolism, Fibrinolytic Agents isolation & purification, Fibrinolytic Agents metabolism, Polychaeta enzymology, Serine Proteases isolation & purification, Serine Proteases metabolism

Abstract

Ischemic stroke can result from blockage of blood vessels, forming fibrin clots in the body and causing irreparable brain damage. Remedial thrombolytic agents or anticoagulants have been studied; however, because the FDA-approved tissue plasminogen activator has low efficacy and side effects, it is necessary to develop safer and more effective treatment candidates. This study aimed at assessing the fibrinolytic and anticoagulation features of a novel serine protease extracted and purified from Diopatra sugokai , a polychaeta that inhabits tidal flats. The purified serine protease was obtained through ammonium sulfate precipitation, affinity chromatography, and ion-exchange chromatography. Its molecular size was identified via SDS-PAGE. To characterize its enzymatic activities, the protease activity at various pH and temperatures, and in the presence of various inhibitors, was measured via azocasein assay. Its fibrinolytic activity and anticoagulant effect were assessed by fibrin zymography, fibrin plate assay, and fibrinogenolytic activity assays. The novel 38 kDa serine protease had strong indirect thrombolytic activity rather than direct activity over broad pH (4-10) and temperature (37°C-70°C) ranges. In addition, the novel serine protease exhibited anticoagulant activity by degrading the α-, β-, and γ-chains of fibrinogen. In addition, it did not produce cytotoxicity in endothelial cells. Therefore, this newly isolated serine protease is worthy of further investigation as a novel alkaline serine protease for thrombolytic therapy against brain ischemia.

Published

2018

16. How nature tunes isoenzyme activity in the multifunctional catalytic globin dehaloperoxidase from Amphitrite ornata.

Author

Carey LM, Gavenko R, Svistunenko DA, and Ghiladi RA

Subjects

Amino Acid Substitution, Animals, Crystallography, X-Ray, Hemoglobins genetics, Hemoglobins metabolism, Isoenzymes chemistry, Isoenzymes genetics, Isoenzymes metabolism, Mutation, Missense, Peroxidase genetics, Peroxidase metabolism, Polychaeta genetics, Protein Domains, Hemoglobins chemistry, Peroxidase chemistry, Polychaeta enzymology

Abstract

The coelomic hemoglobin of Amphitrite ornata, termed dehaloperoxidase (DHP), is the first known multifunctional catalytic globin to possess biologically-relevant peroxidase and peroxygenase activities. Although the two isoenzymes of DHP, A and B, differ in sequence by only 5 amino acids out of 137 residues, DHP B consistently exhibits a greater activity than isoenzyme A. To delineate the contributions of each amino acid substitution to the activity of either isoenzyme, the substitutions of the five amino acids were systematically investigated, individually and in combination, using 22 mutants. Biochemical assays and mechanistic studies demonstrated that the mutants that only contained the I9L substitution showed increased i) k cat values (peroxidase activity), ii) 5-Br-indole conversion and binding affinity (peroxygenase activity), and iii) rate of Compound ES formation (enzyme activation). Whereas the X-ray structures of the oxyferrous forms of DHP B (L9I) (1.96Å), DHP A (I9L) (1.20Å), and WT DHP B (1.81Å) showed no significant differences, UV-visible spectroscopy (A Soret /A 380 ratio) revealed that the I9L substitution increased the 5-coordinate high-spin heme population characterized by the "open" conformation (i.e., distal histidine swung out of the pocket), which likely favors substrate binding. The positioning of the distal histidine closer to the heme cofactor in the solution state also appears to facilitate activation of DHP via the Compound ES intermediate. Taken together, the studies undertaken here shed light on the structure-function relationship in dehaloperoxidase, but also help to establish the foundation for understanding how enzymatic activity can be tuned in isoenzymes of a multifunctional catalytic globin., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2018

17. A study of genotoxicity and oxidative stress induced by mercuric chloride in the marine polychaete Perinereis aibuhitensis.

Author

Zhang LJ, Li Y, Chen P, Li XM, Chen YG, Hang YY, and Gong WJ

Subjects

Animals, Gene Expression Regulation, Enzymologic drug effects, Glutathione Peroxidase metabolism, Micronucleus Tests, Oxidative Stress, Polychaeta drug effects, Polychaeta enzymology, Superoxide Dismutase metabolism, Water Pollutants, Chemical toxicity, DNA Damage, Mercuric Chloride toxicity, Polychaeta genetics

Abstract

The marine polychaete worm Perinereis aibuhitensis was used to study the genotoxic effects of mercuric chloride by means of the comet assay and micronucleus (MN) test. P. aibuhitensis was subjected in vivo to two different concentrations of mercuric chloride (0.05mgL -1 and 0.5mgL -1 ) for 96h. The comet assay of coelomocytes demonstrated that TailDNA% values increased with extended exposure to or increased concentrations of HgCl 2 (p<0.01). The frequency of MNs was the highest in the treatment with 96h of exposure at all concentrations (p<0.01). The genotoxic effect of HgCl 2 was both dose- and time-dependent in exposed P. aibuhitensis. The activities of the antioxidant enzymes, superoxide dismutase (SOD) and glutathione peroxidases (GPx) were also estimated. Significant variations in antioxidant enzyme activities depended on the sampling time and the concentrations of mercuric chloride. Compared with the control, the activities of the antioxidant enzymes (SOD and GPx) were elevated at the lower concentration of mercuric chloride (0.05mg L -1 ) (p<0.05) for shorter exposure periods (24h and 72h). At the higher concentration of mercury (0.5mgL -1 ), the activities of GPx and SOD were inhibited; no variation was observed. These results proved that the use of the comet assay and MN test in coelomocytes of P. aibuhitensis is appropriate for determining the levels of DNA damage and that P. aibuhitensis is a species that is sensitive to mercury pollutants. This species may be considered a suitable candidate for monitoring marine heavy metal pollution., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2017

18. Expression and characterization of recombinant bifunctional enzymes with glutathione peroxidase and superoxide dismutase activities.

Author

Guan T, Song J, Wang Y, Guo L, Yuan L, Zhao Y, Gao Y, Lin L, Wang Y, and Wei J

Subjects

Animals, Antioxidants metabolism, Cloning, Molecular, Escherichia coli genetics, Escherichia coli metabolism, Gene Expression, Genetic Vectors chemistry, Genetic Vectors metabolism, Glutathione Peroxidase genetics, Glutathione Peroxidase metabolism, Humans, Hydrogen Peroxide metabolism, Kinetics, Models, Molecular, Polychaeta chemistry, Polychaeta enzymology, Protein Conformation, alpha-Helical, Protein Conformation, beta-Strand, Protein Interaction Domains and Motifs, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Substrate Specificity, Superoxide Dismutase genetics, Superoxide Dismutase metabolism, Superoxides metabolism, Glutathione Peroxidase GPX1, Antioxidants chemistry, Glutathione Peroxidase chemistry, Hydrogen Peroxide chemistry, Recombinant Fusion Proteins chemistry, Superoxide Dismutase chemistry, Superoxides chemistry

Abstract

To balance the production and decomposition of reactive oxygen species, living organisms have generated antioxidant enzymes and non-enzymatic antioxidant defense systems. Glutathione peroxidase (GPx) and superoxide dismutase (SOD) are two important antioxidant enzymes. Apart from their catalytic functions, they protect each other, resulting in more efficient removal of reactive oxygen species, protection of cells against injury, and maintenance of the normal metabolism of reactive oxygen species. SOD catalyzes the dismutation of the superoxide anion (O 2 •- ) to oxygen (O 2 ) and hydrogen peroxide (H 2 O 2 ). H 2 O 2 is then detoxified to water by GPx. In this study, human GPx1 Ser and the Alvinella pompejana SOD (ApSOD) gene were used to design and generate several recombinant proteins with both GPx and SOD activities by combining traditional fusion protein technology, a cysteine auxotrophic expression system, and a single protein production (SPP) system. Among the fusion proteins, Se-hGPx1 Ser -L-ApSOD exhibited the highest SOD and GPx activities. Additional research was conducted to better understand the properties of Se-hGPx1 Ser -L-ApSOD. The synergism of Se-hGPx1 Ser -L-ApSOD was evaluated by using an in vitro model. This research may facilitate future studies on the cooperation and catalytic mechanisms of GPx and SOD. We believe that the bifunctional enzyme has potential applications as a potent antioxidant., (Copyright © 2017 Elsevier Inc. All rights reserved.)

Published

2017

19. A Novel ω3-Desaturase in the Deep Sea Giant Tubeworm Riftia pachyptila.

Author

Liu H, Wang H, Cai S, and Zhang H

Subjects

Animals, Fatty Acid Desaturases genetics, Fatty Acids, Omega-3 biosynthesis, Gene Expression, Hydrothermal Vents, Polychaeta genetics, Saccharomyces cerevisiae, Fatty Acid Desaturases metabolism, Polychaeta enzymology

Abstract

One paradox of the trophic biochemistry of the deep sea giant tubeworm Riftia pachyptila, endemic to hydrothermal vent sites and nourished by polyunsaturated fatty acid (PUFA) deficiency chemolitoautotrophic sulfide-oxidizing bacteria, is the source of their PUFAs. Biosynthesis of PUFA starts with two precursors C18:2n-6 and C18:3n-3, which cannot be biosynthesized by most animals due to lack of ω6- and ω3-desaturase; thus, C18:2n-6 and C18:3n-3 are generally essential fatty acids for animals. Here, we characterized a gene derived from the R. pachyptila located by hydrothermal vent, which encoded a novel ω3-desaturase (Rp3Fad). The gene was identified by searching the R. pachyptila transcriptome database using known ω3-desaturases, and its predicted protein showed 37-45% identical to ω3-desaturases of fungus and microalgae, and only 31% identitical to nematode Caenorhabditis elegans ω3-desaturase. Expression in yeast Saccharomyces cerevisiae showed that the Rp3Fad could desaturate C18:2n-6 and C18:3n-6 into C18:3n-3 and C18:4n-3, respectively, displaying a Δ15 activity similar to plant ω3-desaturase, but it showed no activity towards C20 n-6 PUFA substrates, differing from the well-characterized C. elegans ω3-desaturases. Δ5, Δ6, Δ8, and Δ12 activity were also tested, resulting in no corresponding production. The function of ω3-desaturase identified in R. pachyptila could produce C18:3n - 3 used in synthesis of n - 3 series PUFAs, suggesting an adaption to PUFA deficiency environment in deep sea hydrothermal vent.

Published

2017

20. Purification of serine protease from polychaeta, Lumbrineris nipponica, and assessment of its fibrinolytic activity.

Author

Yeon SJ, Chung GY, Hong JS, Hwang JH, and Shin HS

Subjects

Amino Acid Sequence genetics, Animals, Fibrin chemistry, Fibrin genetics, Fibrinolytic Agents chemistry, Fibrinolytic Agents therapeutic use, Polychaeta enzymology, Serine Proteases chemistry, Serine Proteases therapeutic use, Brain Ischemia drug therapy, Fibrinolytic Agents isolation & purification, Serine Proteases isolation & purification, Stroke drug therapy

Abstract

Ischemic stroke and cardiovascular disease can occur from blockage of blood vessels by fibrin clots formed naturally in the body. Therapeutic drugs of anticoagulant or thrombolytic agents have been studied; however, various problems have been reported such as side effects and low efficacy. Thus, development of new candidates that are more effective and safe is necessary. The objective of this study is to evaluate fibrinolytic activity, anti-coagulation, and characterization of serine protease purified from Lumbrineris nipponica, polychaeta, for new thrombolytic agents. In the present study, we isolated and identified a new fibrinolytic serine protease from L. nipponica. The N-terminal sequence of the identified serine protease was EAMMDLADQLEQSLN, which is not homologous with any known serine protease. The size of the purified serine protease was 28 kDa, and the protein purification yield was 12.7%. The optimal enzyme activity was observed at 50°C and pH 2.0. A fibrin plate assay confirmed that indirect fibrinolytic activity of the purified serine protease was higher than that of urokinase-PA, whereas direct fibrinolytic activity, which causes bleeding side effects, was relatively low. The serine protease did not induce any cytotoxicity toward the endothelial cell line. In addition, anticoagulant activity was verified by an in vivo DVT animal model system. These results suggest that serine protease purified from L. nipponica has the potential to be an alternative fibrinolytic agent for the treatment of thrombosis and use in various biomedical applications.

Published

2017

21. Interaction of Azole-Based Environmental Pollutants with the Coelomic Hemoglobin from Amphitrite ornata: A Molecular Basis for Toxicity.

Author

McCombs NL, Moreno-Chicano T, Carey LM, Franzen S, Hough MA, and Ghiladi RA

Subjects

Amino Acid Motifs, Animals, Benzimidazoles chemistry, Benzimidazoles toxicity, Catalytic Domain, Computational Biology, Environmental Pollutants chemistry, Environmental Pollutants toxicity, Enzyme Inhibitors chemistry, Enzyme Inhibitors metabolism, Enzyme Inhibitors toxicity, Fungicides, Industrial chemistry, Fungicides, Industrial metabolism, Fungicides, Industrial toxicity, Hemoglobins antagonists & inhibitors, Hemoglobins chemistry, Hydrogen Bonding, Hydrophobic and Hydrophilic Interactions, Imidazoles chemistry, Imidazoles toxicity, Indazoles chemistry, Indazoles metabolism, Indazoles toxicity, Isoenzymes antagonists & inhibitors, Isoenzymes chemistry, Isoenzymes metabolism, Kinetics, Ligands, Peroxidases antagonists & inhibitors, Peroxidases chemistry, Pesticides chemistry, Pesticides metabolism, Pesticides toxicity, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins metabolism, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Triazoles chemistry, Triazoles toxicity, Benzimidazoles metabolism, Environmental Pollutants metabolism, Hemoglobins metabolism, Imidazoles metabolism, Models, Molecular, Peroxidases metabolism, Polychaeta enzymology, Triazoles metabolism

Abstract

The toxicities of azole pollutants that have widespread agricultural and industrial uses are either poorly understood or unknown, particularly with respect to how infaunal organisms are impacted by this class of persistent organic pollutant. To identify a molecular basis by which azole compounds may have unforeseen toxicity on marine annelids, we examine here their impact on the multifunctional dehaloperoxidase (DHP) hemoglobin from the terebellid polychaete Amphitrite ornata. Ultraviolet-visible and resonance Raman spectroscopic studies showed an increase in the six-coordinate low-spin heme population in DHP isoenzyme B upon binding of imidazole, benzotriazole, and benzimidazole (K d values of 52, 82, and 110 μM, respectively), suggestive of their direct binding to the heme-Fe. Accordingly, atomic-resolution X-ray crystal structures, supported by computational studies, of the DHP B complexes of benzotriazole (1.14 Å), benzimidazole (1.08 Å), imidazole (1.08 Å), and indazole (1.12 Å) revealed two ligand binding motifs, one with direct ligand binding to the heme-Fe, and another in which the ligand binds in the hydrophobic distal pocket without coordinating the heme-Fe. Taken together, the results demonstrate a new mechanism by which azole pollutants can potentially disrupt hemoglobin function, thereby improving our understanding of their impact on infaunal organisms in marine and aquatic environments.

Published

2017

22. Cu/Zn superoxide dismutase (SOD) and catalase (CAT) response to crude oil exposure in the polychaete Perinereis aibuhitensis.

Author

Zhao H, Li W, Zhao X, Li X, Yang D, Ren H, and Zhou Y

Subjects

Animals, Catalase metabolism, DNA, Complementary genetics, Gene Expression Regulation, Enzymologic drug effects, Polychaeta enzymology, Polychaeta genetics, Superoxide Dismutase-1 metabolism, Catalase genetics, Petroleum toxicity, Polychaeta drug effects, Superoxide Dismutase-1 genetics, Water Pollutants, Chemical toxicity

Abstract

Cu/Zn superoxide dismutase (SOD) and catalase (CAT) cDNAs from the polychaete Perinereis aibuhitensis were cloned and characterized in order to investigate the relationship between crude oil exposure and stress response in this worm. The full length of PaSOD was 870 bp and PaCAT was 1967 bp encoding 150 and 506 amino acids, respectively. Gene expression and enzyme activity of Cu/Zn SOD and CAT in response to crude oil contaminated soil (500, 1500, and 3000 mg/kg) were measured. The results showed that expression of the CAT gene and enzyme activity in P. aibuhitensis was positively correlated to the concentration of crude oil and reached a maximum at 15 days of exposure to 3000 mg/kg crude oil. The expression of the SOD gene and enzyme activity of SOD in P. aibuhitensis also increased during exposure to crude oil and reached a maximum at 10 days of exposure to 3000 mg/kg crude oil. These results indicated that SOD and CAT are important for maintaining the balance of cellular metabolism and protecting P. aibuhitensis from crude oil toxicity.

Published

2017

23. Suitability of cholinesterase of polychaete Diopatra neapolitana as biomarker of exposure to pesticides: In vitro characterization.

Author

Mennillo E, Casu V, Tardelli F, De Marchi L, Freitas R, and Pretti C

Subjects

Animals, Biomarkers metabolism, Dose-Response Relationship, Drug, Hydrolysis, Kinetics, Native Polyacrylamide Gel Electrophoresis, Polychaeta enzymology, Substrate Specificity, Temperature, Carbamates toxicity, Cholinesterase Inhibitors toxicity, Cholinesterases metabolism, Environmental Monitoring methods, Pesticides toxicity, Polychaeta drug effects, Water Pollutants, Chemical toxicity

Abstract

Cholinesterases of Diopatra neapolitana were characterized for their activity in whole body and different body segments (apical, intermediate, posterior), substrate affinity (acetyl-, butyryl-, propionylthiocholine), kinetic parameters (K m and V max ) and in vitro response to model inhibitors (eserine hemisulfate, isoOMPA, BW284C51) and carbamates (carbofuran, methomyl, aldicarb and carbaryl). Results showed that the rate of hydrolysis for acetyl- and propionylthiocholine was higher in the posterior segment than the apical/intermediate segments and whole body. Cholinesterases of D. neapolitana showed a substrate preference for acetylthiocholine followed by propionylthiocholine; butyrylthioline was poorly hydrolyzed indicating, together with the absence of inhibition by the specific inhibitor and the absence of reactive bands in native electrophoresis, a lack of an active butyrylcholinesterase, differently than that observed in other Annelida species. The degree of inhibition by selected carbamates of cholinesterase activity with propionylthiocholine as substrate was higher than that observed with ATChI-ChE activity; aldicarb showed the highest inhibitory effect., (Copyright © 2016 Elsevier Inc. All rights reserved.)

Published

2017

24. Expression and Localization of Carbonic Anhydrase Genes in the Serpulid Polychaete Hydroides elegans.

Author

Batzel G, Nedved BT, and Hadfield MG

Subjects

Animals, Calcium Carbonate, Evolution, Molecular, Gene Expression Regulation, Enzymologic, Phylogeny, Polychaeta classification, Carbonic Anhydrases genetics, Polychaeta enzymology, Polychaeta genetics

Abstract

The metalloenzyme, carbonic anhydrase (CA), catalyzes the reversible hydration of carbon dioxide into bicarbonate, and is responsible for biomineralization processes in animals. In the Annelida, the marine worms in the family Serpulidae are typified by the construction of calcium carbonate tubes. Hydroides elegans, a common member of warmwater biofouling communities around the world, provides an outstanding model for studies of calcification. To better understand the molecular process of biomineralization in H. elegans, we searched transcriptomes for CA genes at several life-history stages. Twelve CA genes were recovered in the transcriptomes. Whole mount in situ hybridization was performed for two of those genes on larvae and calcifying juveniles. A cytosolic CA isoform, HeCA1, and a secreted CA isoform, HeCA2, were expressed within the collar segment corresponding to the location of glands involved in formation of the calcified tube. Expression of these genes within collar segment tissues supports the role of CAs in generating bicarbonate for biomineralization processes. A phylogenetic tree of the α-CA gene family was constructed to increase understanding of CA-gene evolution within the family and its relationship to CA genes among the Metazoa.

Published

2016

25. Role of proteasomes in non-specific immune response of marine annelids.

Author

Stanovova MV, Erokhov PA, Gornostaev NG, Mikhailov VS, and Lyupina YV

Subjects

Animals, Blotting, Western, Electrophoresis, HSP70 Heat-Shock Proteins metabolism, Lipopolysaccharides, Polychaeta enzymology, Polychaeta immunology, Proteasome Endopeptidase Complex metabolism

Abstract

We investigated functioning of proteasomes and chaperones in Arenicola marina coelomocytes in conditions of lipopolysaccharide-induced inflammation. We observed the increase of chymotrypsin-like proteasome activity in coelomocytes 1 h after induction. Amount of proteasome subunits alpha- and beta-5 types increased as well. We also detected appearance of a new form of Hsp70 chaperone in infected coelomocytes. Our results allow us to consider the changes in proteasome structure and induction of chaperones as principle mechanisms in stress adaptation and defensive reactions development in annelids.

Published

2016

26. Vanadium-Binding Ability of Nucleoside Diphosphate Kinase from the Vanadium-Rich Fan Worm, Pseudopotamilla occelata.

Author

Yamaguchi N, Yoshinaga M, Kamino K, and Ueki T

Subjects

Animals, Carrier Proteins, Chromatography, Affinity, Epidermis enzymology, Nucleoside-Diphosphate Kinase metabolism, Polychaeta enzymology, Vanadium metabolism

Abstract

Polychaete fan worms and ascidians accumulate high levels of vanadium ions. Several vanadiumbinding proteins, known as vanabins, have been found in ascidians. However, no vanadium-binding factors have been isolated from the fan worm. In the present study, we sought to identify vanadiumbinding proteins in the branchial crown of the fan worm using immobilized metal ion affinity chromatography. A nucleoside diphosphate kinase (NDK) homolog was isolated and determined to be a vanadium-binding protein. Kinase activity of the NDK homologue, PoNDK, was suppressed by the addition of V(IV), but was unaffected by V(V). The effect of V(IV) on PoNDK precedes its activation by Mg(II). This is the first report to describe the relationship between NDK and V(IV). PoNDK is located in the epidermis of the branchial crown, and its distribution is very similar to that of vanadium. These results suggest that PoNDK is associated with vanadium accumulation and metabolism in P. occelata.

Published

2016

27. Nonmicrobial Nitrophenol Degradation via Peroxygenase Activity of Dehaloperoxidase-Hemoglobin from Amphitrite ornata.

Author

McCombs NL, D'Antonio J, Barrios DA, Carey LM, and Ghiladi RA

Subjects

Animals, Catalysis, Hydrogen Peroxide metabolism, Nitrophenols, Oxidation-Reduction, Hemoglobins metabolism, Mixed Function Oxygenases metabolism, Oxygen metabolism, Peroxidases metabolism, Polychaeta enzymology

Abstract

The marine hemoglobin dehaloperoxidase (DHP) from Amphitrite ornata was found to catalyze the H2O2-dependent oxidation of nitrophenols, an unprecedented nonmicrobial degradation pathway for nitrophenols by a hemoglobin. Using 4-nitrophenol (4-NP) as a representative substrate, the major monooxygenated product was 4-nitrocatechol (4-NC). Isotope labeling studies confirmed that the O atom incorporated was derived exclusively from H2O2, indicative of a peroxygenase mechanism for 4-NP oxidation. Accordingly, X-ray crystal structures of 4-NP (1.87 Å) and 4-NC (1.98 Å) bound to DHP revealed a binding site in close proximity to the heme cofactor. Peroxygenase activity could be initiated from either the ferric or oxyferrous states with equivalent substrate conversion and product distribution. The 4-NC product was itself a peroxidase substrate for DHP, leading to the secondary products 5-nitrobenzene-triol and hydroxy-5-nitro-1,2-benzoquinone. DHP was able to react with 2,4-dinitrophenol (2,4-DNP) but was unreactive against 2,4,6-trinitrophenol (2,4,6-TNP). pH dependence studies demonstrated increased reactivity at lower pH for both 4-NP and 2,4-DNP, suggestive of a pH effect that precludes the reaction with 2,4,6-TNP at or near physiological conditions. Stopped-flow UV-visible spectroscopic studies strongly implicate a role for Compound I in the mechanism of 4-NP oxidation. The results demonstrate that there may be a much larger number of nonmicrobial enzymes that are underrepresented when it comes to understanding the degradation of persistent organic pollutants such as nitrophenols in the environment.

Published

2016

28. [The expression of phenylalanine hydroxylase in the brain of ragworm Neanthes japonica (Polychaeta, Annelida)].

Author

Ren G, Dong Z, Liu C, Liu Y, Luan Z, Liu Q, Bao X, and Wang S

Subjects

Animals, Blotting, Western, Escherichia coli metabolism, Phenylalanine Hydroxylase genetics, Polychaeta genetics, Brain enzymology, Phenylalanine Hydroxylase metabolism, Polychaeta enzymology

Abstract

Phenylalanine hydroxylase (PAH) is a member of aromatic amino acid hydroxylase (AAAHs) family, and catalyze phenylalanine (Phe) into tyrosine (Tyr). Using immunological and RT-PCR methods to prove the existence of phenylalanine hydroxylase (PAH) gene in the brain of Neanthes japonica in protein and nucleic acid level. Using Western blotting to detect the pah immunogenicity of Neanthes japonica. Making paraffin sections and using immunohistochemical technique to identify the presence and distribution of the phenylalanine hydroxylase gene in the brain of Neanthes japonica. Clone pah gene from the brain of Neanthes japonica by RT-PCR, constructing plasmid and transferring into E. coli to amplification, picking a single homogeneous colony, double digesting then making sequence and comparing homology. Western blotting results showed that the expression of the protein is present in Neanthes japonica brain, immunohistochemistry technique results showed that phenylalanine hydroxylase mainly expressed in abdominal of forebrain, dorsal and sides of midbrain. RT-PCR technique results showed that the phenylalanine hydroxylase exist in the brain of Neanthes japonica and has a high homology with others animals. PAH is present in the lower organisms Neanthes japonica, in protein and nucleic acid level. Which provide the foundation for further study the evolution of aromatic amino acid hydroxylase genes in invertebrate.

Published

2016

29. Correlation of heme binding affinity and enzyme kinetics of dehaloperoxidase.

Author

Le P, Zhao J, and Franzen S

Subjects

Animals, Kinetics, Polychaeta enzymology, Protein Binding, Protein Denaturation, Thermodynamics, Heme chemistry, Hemoglobins chemistry, Peroxidases chemistry

Abstract

Chemical and thermal denaturation of dehaloperoxidase-hemoglobin (DHP) was investigated to test the relative stability of isoforms DHP A and DHP B and the H55V mutant of DHP A with respect to heme loss. In thermal denaturation experiments, heme loss was observed at temperatures of 54, 46, and 61 °C in DHP A, DHP B, and H55V, respectively. Guanidinium hydrochloride (GdnHCl)- and urea-induced denaturation was observed at respective concentrations of 1.15 ± 0.01 M DHP A and 1.09 ± 0.02 M DHP B, and 5.19 ± 0.05 M DHP A and 4.12 ± 0.14 M DHP B, respectively. The binding affinity of heme appears to be significantly smaller in both isoforms of DHP than in myoglobins. This observation was corroborated by heme transfer experiments, in which heme was observed to transfer for DHP A and B to horse skeletal muscle myoglobin (HSMb). GdnHCl-induced denaturation suggests a threshold of 1 mM for stabilization by binding of the inhibitor 4-bromophenol (4-BP). Concentrations of 4-BP greater than 1 mM caused destabilization. Urea-induced denaturation showed only destabilizing effects from phenolic ligand binding. Heme transfer experiments from DHP to HSMb further support the hypothesis that the binding of halophenols to DHP facilitates the removal of the heme. Thermal denaturation assessed via UV-visible spectroscopy and that assessed by differential scanning calorimetry (DSC) are both in agreement with chemical denaturation experiments and show that the denaturing abilities of the halophenols improve with the size of the para halogen atom in 4-XP, where X = iodo, bromo, chloro, or fluoro (4-IP > 4-BP > 4-CP > 4-FP), and the number of halo substituents as in 2,4,6-tribromophenol (2,4,6-TBP > 4-BP). DHP B, which differs in five amino acids, is less stable than DHP A with ΔHcal and Tm values of 165.1 kJ/mol and 47.5 °C compared to values of 183.3 kJ/mol and 50.4 °C for DHP B and DHP A, respectively. Kinetic studies verified that DHP B has a catalytic efficiency (kcat/Km) ∼5-6 times greater than that of DHP A but showed an increased level of substrate inhibition in DHP B for both 2,4,6-TCP and 2,4,6-TBP. An inverse correlation between protein stability with respect to heme loss and catalytic efficiency is suggested on the basis of the fact that the heme in DHP B has a stability lower than that of DHP A but a catalytic efficiency higher than that of DHP A.

Published

2014

30. Three novel superoxide dismutase genes identified in the marine polychaete Perinereis nuntia and their differential responses to single and combined metal exposures.

Author

Won EJ, Ra K, Kim KT, Lee JS, and Lee YM

Subjects

Amino Acid Sequence, Animals, Antioxidants metabolism, Base Sequence, Biomarkers metabolism, Ecosystem, Metals metabolism, Metals, Heavy analysis, Metals, Heavy metabolism, Mitochondria metabolism, Molecular Sequence Data, Oceans and Seas, Phylogeny, Polychaeta enzymology, RNA, Messenger metabolism, Superoxide Dismutase metabolism, Environmental Monitoring, Heavy Metal Poisoning, Poisoning metabolism, Polychaeta genetics, Superoxide Dismutase genetics, Water Pollution, Chemical analysis

Abstract

To identify superoxide dismutase (SOD) genes and evaluate their usefulness as potential markers for monitoring metal toxicity in aquatic environment, we cloned, sequenced, and characterized 3 SOD genes (Cu/Zn-SOD1, Cu/Zn-SOD2, and Mn-SOD) from the marine polychaete Perinereis nuntia. The accumulated metal contents and expressions of 3 SOD genes were compared after exposure to single and combinations of heavy metals, As, Ni, and Pb. The deduced amino acid sequences of the 3 SODs had evolutionary conserved domains, such as metal binding sites, and signature sequences. The phylogenetic analysis revealed that Cu/Zn-SOD1, Cu/Zn-SOD2, and Mn-SOD were clustered with extracellular Cu/Zn-SOD, intracellular Cu/Zn-SOD and mitochondrial Mn-SOD, respectively, of other species. The accumulated contents of Ni and Pb increased significantly in a time - dependent manner after exposure to both single and combination of the metals. However, the concentration of As did not change significantly in the exposure test. The quantitative real-time polymerase chain reaction (PCR) array showed that the 3 SOD genes had differential expression patterns depending on the exposure condition. The expression of all SODs mRNAs was significantly elevated in response to Pb alone and in combination with As. The mRNA level of Cu/Zn-SOD1 was the highest after exposure to Pb alone, while that of Mn-SOD was remarkably enhanced after exposure to a combination of As and Pb. Exposure to Ni alone rapidly elevated the expression of Cu/Zn-SOD1 and Mn-SOD mRNA, which then gradually decreased. Exposure to As had no significant effect on the modulation of any of the SOD genes of P. nuntia. These results suggest that all SOD genes might play important roles in cellular protection as antioxidant enzymes against heavy metal toxicity via different modes of action in P. nuntia and might have the potential to act as indicators in an environment containing a mixture of metals., (Copyright © 2014 Elsevier Inc. All rights reserved.)

Published

2014

31. Peroxygenase and oxidase activities of dehaloperoxidase-hemoglobin from Amphitrite ornata.

Author

Barrios DA, D'Antonio J, McCombs NL, Zhao J, Franzen S, Schmidt AC, Sombers LA, and Ghiladi RA

Subjects

Animals, Catalytic Domain, Hemoglobins chemistry, Indoles chemistry, Indoles metabolism, Models, Molecular, Oxygen chemistry, Oxygen Consumption, Oxygen Radioisotopes, Protein Conformation, Hemoglobins metabolism, Mixed Function Oxygenases metabolism, Oxidoreductases metabolism, Polychaeta enzymology

Abstract

The marine globin dehaloperoxidase-hemoglobin (DHP) from Amphitrite ornata was found to catalyze the H2O2-dependent oxidation of monohaloindoles, a previously unknown class of substrate for DHP. Using 5-Br-indole as a representative substrate, the major monooxygenated products were found to be 5-Br-2-oxindole and 5-Br-3-oxindolenine. Isotope labeling studies confirmed that the oxygen atom incorporated was derived exclusively from H2O2, indicative of a previously unreported peroxygenase activity for DHP. Peroxygenase activity could be initiated from either the ferric or oxyferrous states with equivalent substrate conversion and product distribution. It was found that 5-Br-3-oxindole, a precursor of the product 5-Br-3-oxindolenine, readily reduced the ferric enzyme to the oxyferrous state, demonstrating an unusual product-driven reduction of the enzyme. As such, DHP returns to the globin-active oxyferrous form after peroxygenase activity ceases. Reactivity with 5-Br-3-oxindole in the absence of H2O2 also yielded 5,5'-Br2-indigo above the expected reaction stoichiometry under aerobic conditions, and O2-concentration studies demonstrated dioxygen consumption. Nonenzymatic and anaerobic controls both confirmed the requirements for DHP and molecular oxygen in the catalytic generation of 5,5'-Br2-indigo, and together suggest a newly identified oxidase activity for DHP.

Published

2014

32. Molecular cloning, expression, and anti-tumor activity of a novel serine protease from Arenicola cristata.

Author

Zhao C and Ju J

Subjects

Amino Acid Sequence, Animals, Base Sequence, Cloning, Molecular, DNA Primers, DNA, Complementary, Mice, Mice, Inbred BALB C, Molecular Sequence Data, Open Reading Frames, Polymerase Chain Reaction, Sequence Homology, Amino Acid, Serine Proteases genetics, Polychaeta enzymology, Serine Proteases metabolism

Abstract

Arenicola cristata, a marine annelid, is a well-known and prized traditional Chinese medicine. However, the serine protease gene of A. cristata has not been cloned yet. In this study, a novel protease of A. cristata was cloned, sequenced, and expressed in Escherichia coli, and the functions of this recombinant protease were also investigated. The whole complementary DNA (cDNA) of this novel protease was of 980 bp in length and consisted of an open reading frame of 861 bp encoding 286 aa. Sequence analysis of the deduced amino acid sequence revealed that the protease belongs to the serine protease family. The active enzyme of the proposed A. cristata protease is composed of a signal peptide, a propeptide, and a mature polypeptide. The molecular weight of the recombinant mature protein was ~26 kDa after over-expression in E. coli. The recombinant protein significantly inhibited cell growth and induced cell apoptosis of esophageal squamous cell carcinoma (ESCC) in vitro, and reduced tumorigenicity in vivo. Furthermore, administration of the recombinant protein led to the activation of caspase-9 as well as down-regulation of Mcl-1 and Bcl-2. Taken together, our findings indicated that the recombinant serine protease of A. cristata could inhibit ESCC cell growth by mitochondrial apoptotic pathway and might act as a potential pharmacological agent for ESCC therapy., (© The Author 2014. Published by ABBS Editorial Office in association with Oxford University Press on behalf of the Institute of Biochemistry and Cell Biology, Shanghai Institutes for Biological Sciences, Chinese Academy of Sciences.)

Published

2014

33. Influence of heme environment structure on dioxygen affinity for the dual function Amphitrite ornata hemoglobin/dehaloperoxidase. Insights into the evolutional structure-function adaptations.

Author

Sun S, Sono M, Wang C, Du J, Lebioda L, and Dawson JH

Subjects

Animals, Crystallography, X-Ray, Heme metabolism, Models, Molecular, Myoglobin chemistry, Peroxidases chemistry, Polychaeta chemistry, Polychaeta metabolism, Protein Conformation, Sperm Whale metabolism, Heme chemistry, Myoglobin metabolism, Oxygen metabolism, Peroxidases metabolism, Polychaeta enzymology

Abstract

Sea worm, Amphitrite ornata, has evolved its globin (an O(2) carrier) also to serves as a dehaloperoxidase (DHP) to detoxify haloaromatic pollutants generated by competing species. A previous mutagenesis study by our groups on both DHP and sperm whale myoglobin (SW Mb) revealed some structural factors that influence the dehaloperoxidase activities (significantly lower for Mb) of both proteins. Using an isocyanide/O(2) partition constant measurement method in this study, we have examined the effects of these structural factors on the O(2) equilibrium constants (KO2) of DHP, SW Mb, and their mutants. A clear trend of decreasing O(2) affinity and increasing catalytic activity along with the increase in the distal His N(ε)-heme iron distance is observed. An H93K/T95H Mb double mutant mimicking the DHP proximal His positioning exhibited markedly enhanced O(2) affinity, confirming the essential effect of proximal His rotation on the globin function of DHP. For DHP, the L100F, T56G and M86E variants showed the effects of distal volume, distal His flexibility and proximal electronic push, respectively, on the O(2) affinity. This study provides insights into how DHP has evolved its heme environment to gain significantly enhanced peroxidase capability without compromising its primary function as an O(2) carrier., (Copyright © 2014 Elsevier Inc. All rights reserved.)

Published

2014

34. The dynamics of alkaline phosphatase activity during operculum regeneration in the polychaete Pomatoceros lamarckii.

Author

Szabó R and Ferrier DE

Subjects

Alkaline Phosphatase metabolism, Amino Acid Sequence, Animals, Antinematodal Agents pharmacology, Biological Evolution, Calcification, Physiologic physiology, Levamisole pharmacology, Molecular Sequence Data, Sequence Alignment, Alkaline Phosphatase genetics, Polychaeta enzymology, Polychaeta growth & development, Regeneration physiology

Abstract

Alkaline phosphatase enzymes are found throughout the living world and fulfil a variety of functions. They have been linked to regeneration, stem cells and biomineralisation in a range of animals. Here we describe the pattern of alkaline phosphatase activity in a spiralian appendage, the operculum of the serpulid polychaete Pomatoceros lamarckii. The P. lamarckii operculum is reinforced by a calcified opercular plate and is capable of rapid regeneration, making it an ideal model system to study these key processes in annelids. Alkaline phosphatase activity is present in mesodermal tissues of both intact and regenerating opercular filaments, in a strongly regionalised pattern correlated with major morphological features. Based on the lack of epidermal activity and the broad distribution of staining in mesodermal tissues, calcification- or stem cell-specific roles are unlikely. Transcriptomic data reveal that at least four distinct genes contribute to the detected activity. Opercular alkaline phosphatase activity is sensitive to levamisole. Phylogenetic analysis of metazoan alkaline phosphatases indicates homology of the P. lamarckii sequences to other annelid alkaline phosphatases, and shows that metazoan alkaline phosphatase evolution was characterised by extensive lineage-specific duplications.

Published

2014

35. Characteristics and function of sulfur dioxygenase in Echiuran worm Urechis unicinctus.

Author

Zhang L, Liu X, Liu J, and Zhang Z

Subjects

Amino Acid Sequence, Animals, Base Sequence, Biocatalysis, Cloning, Molecular, DNA, Complementary genetics, Dioxygenases genetics, Models, Molecular, Molecular Sequence Data, Mutation, Phylogeny, Protein Refolding, Protein Structure, Secondary, Protein Structure, Tertiary, Dioxygenases chemistry, Dioxygenases metabolism, Polychaeta enzymology

Abstract

Background: Sulfide is a common toxin to animals and is abundant in coastal and aquatic sediments. Sulfur dioxygenase (SDO) is thought to be the key enzyme involved in sulfide oxidation in some organisms. The echiuran worm, Urechis unicinctus, inhabits coastal sediment and tolerates high concentrations of sulfide. The SDO is presumably important for sulfide tolerance in U. unicinctus., Results: The full-length cDNA of SDO from the echiuran worm U. unicinctus, proven to be located in the mitochondria, was cloned and the analysis of its sequence suggests that it belongs to the metallo-β-lactamase superfamily. The enzyme was produced using an E. coli expression system and the measured activity is approximately 0.80 U mg protein(-1). Furthermore, the expression of four sub-segments of the U. unicinctus SDO was accomplished leading to preliminary identification of functional domains of the enzyme. The identification of the conserved metal I (H113, H115, H169 and D188), metal II (D117, H118, H169 and H229) as well as the potential glutathione (GSH) (R197, Y231, M279 and I283) binding sites was determined by enzyme activity and GSH affinity measurements. The key residues responsible for SDO activity were identified by analysis of simultaneous mutations of residues D117 and H118 located close to the metal II binding site., Conclusion: The recombinant SDO from U. unicinctus was produced, purified and characterized. The metal binding sites in the SDO were identified and Y231 recognized as the mostly important amino acid residue for GSH binding. Our results show that SDO is located in the mitochondria where it plays an important role in sulfide detoxification of U. unicinctus.

Published

2013

36. The regulatory implications of hydroquinone for the multifunctional enzyme dehaloperoxidase-hemoglobin from Amphitrite ornata.

Author

Zhao J, Zhao J, and Franzen S

Subjects

Animals, Chlorophenols metabolism, Hemoglobins chemistry, Hydrogen Peroxide metabolism, Models, Molecular, Multifunctional Enzymes chemistry, Oxidation-Reduction, Peroxidases chemistry, Phenols metabolism, Polychaeta chemistry, Polychaeta metabolism, Hemoglobins metabolism, Hydroquinones metabolism, Multifunctional Enzymes metabolism, Peroxidases metabolism, Polychaeta enzymology

Abstract

Hydroquinone (H2Q) has been observed to compete with the oxidation of substrates 2,4,6-tribromophenol (2,4,6-TBP) and 2,4,6-trichlorophenol (2,4,6-TCP) catalyzed by the dehaloperoxidase-hemoglobin (DHP) from Amphitrite ornata in the presence of H2O2. This competition is observed as a lag phase during which H2Q is preferentially oxidized to 1,4-benzoquinone (1,4-BQ) while totally inhibiting either 2,4,6-TBP or 2,4,6-TCP oxidation. The inhibition by H2Q is distinct from that of the native competitive inhibitor 4-bromophenol (4-BP) since H2Q is itself oxidized and its product 1,4-BQ is not an inhibitor. Thus, once H2Q is completely consumed, the inhibition is removed, and normal substrate turnover is initiated, which explains the lag phase. To probe the mechanism of lag phase, the reactions between H2Q and DHP were both studied both in the presence and in the absence of H2O2. The reversible reactions between ferric/oxyferrous DHP A and H2Q/1,4-BQ are shown to involve a proton-coupled electron transfer (PCET) mechanism, where the distal histidine His(55) serves as the proton acceptor. The pKa of the distal histidine His(55) has been determined by resonance Raman spectroscopy in order to corroborate its involvement in this mechanism. Consistent with the proposed mechanism, kinetic assays have shown that H2Q serves as a substrate for DHP that follows the Michaelis-Menten kinetics. Unlike H2Q, the product 1,4-BQ has a relatively large Ki value and therefore has negligible inhibition. This study sheds light on understanding the difference between substrate and inhibitor binding sites and regulatory implication for the peroxidase and oxygen-transporter functions in DHP. It also provides information on PCET in DHP, which is important for resolving the switching between the ferric peroxidase catalytic function and the ferrous oxygen transport function.

Published

2013

37. Tyrosyl radicals in dehaloperoxidase: how nature deals with evolving an oxygen-binding globin to a biologically relevant peroxidase.

Author

Dumarieh R, D'Antonio J, Deliz-Liang A, Smirnova T, Svistunenko DA, and Ghiladi RA

Subjects

Animals, Hemoglobins genetics, Hemoglobins metabolism, Oxidation-Reduction, Oxygen metabolism, Peroxidase genetics, Peroxidase metabolism, Peroxidases genetics, Peroxidases metabolism, Protein Binding, Tyrosine chemistry, Tyrosine genetics, Tyrosine metabolism, Adaptation, Physiological, Hemoglobins chemistry, Oxygen chemistry, Peroxidase chemistry, Peroxidases chemistry, Polychaeta enzymology, Tyrosine analogs & derivatives

Abstract

Dehaloperoxidase (DHP) from Amphitrite ornata, having been shown to catalyze the hydrogen peroxide-dependent oxidation of trihalophenols to dihaloquinones, is the first oxygen binding globin that possesses a biologically relevant peroxidase activity. The catalytically competent species in DHP appears to be Compound ES, a reactive intermediate that contains both a ferryl heme and a tyrosyl radical. By simulating the EPR spectra of DHP activated by H2O2, Thompson et al. (Thompson, M. K., Franzen, S., Ghiladi, R. A., Reeder, B. J., and Svistunenko, D. A. (2010) J. Am. Chem. Soc. 132, 17501-17510) proposed that two different radicals, depending on the pH, are formed, one located on either Tyr-34 or Tyr-28 and the other on Tyr-38. To provide additional support for these simulation-based assignments and to deduce the role(s) that tyrosyl radicals play in DHP, stopped-flow UV-visible and rapid-freeze-quench EPR spectroscopic methods were employed to study radical formation in DHP when three tyrosine residues, Tyr-28, Tyr-34, and Tyr-38, were replaced either individually or in combination with phenylalanines. The results indicate that radicals form on all three tyrosines in DHP. Evidence for the formation of DHP Compound I in several tyrosine mutants was obtained. Variants that formed Compound I showed an increase in the catalytic rate for substrate oxidation but also an increase in heme bleaching, suggesting that the tyrosines are necessary for protecting the enzyme from oxidizing itself. This protective role of tyrosines is likely an evolutionary adaptation allowing DHP to avoid self-inflicted damage in the oxidative environment.

Published

2013

38. Binding region of alanopine dehydrogenase predicted by unbiased molecular dynamics simulations of ligand diffusion.

Author

Gohlke H, Hergert U, Meyer T, Mulnaes D, Grieshaber MK, Smits SH, and Schmitt L

Subjects

Alanine metabolism, Amino Acid Substitution, Animals, Binding Sites, Diffusion, Helminth Proteins genetics, Helminth Proteins metabolism, Kinetics, Ligands, Oxidoreductases Acting on CH-NH Group Donors genetics, Oxidoreductases Acting on CH-NH Group Donors metabolism, Polychaeta enzymology, Protein Binding, Protein Structure, Secondary, Protein Structure, Tertiary, Pyruvic Acid metabolism, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Structural Homology, Protein, Substrate Specificity, Alanine chemistry, Helminth Proteins chemistry, Molecular Dynamics Simulation, Oxidoreductases Acting on CH-NH Group Donors chemistry, Polychaeta chemistry, Pyruvic Acid chemistry

Abstract

Opine dehydrogenases catalyze the reductive condensation of pyruvate with L-amino acids. Biochemical characterization of alanopine dehydrogenase from Arenicola marina revealed that this enzyme is highly specific for L-alanine. Unbiased molecular dynamics simulations with a homology model of alanopine dehydrogenase captured the binding of L-alanine diffusing from solvent to a putative binding region near a distinct helix-kink-helix motif. These results and sequence comparisons reveal how mutations and insertions within this motif dictate the L-amino acid specificity.

Published

2013

39. The role of T56 in controlling the flexibility of the distal histidine in dehaloperoxidase-hemoglobin from Amphitrite ornata.

Author

Jiang S, Wright I, Swartz P, and Franzen S

Subjects

Animals, Biocatalysis, Hemoglobins genetics, Histidine genetics, Iron chemistry, Kinetics, Molecular Dynamics Simulation, Mutagenesis, Site-Directed, Peroxidases genetics, Polychaeta enzymology, Recombinant Proteins chemistry, Recombinant Proteins genetics, Spectroscopy, Fourier Transform Infrared, Spectrum Analysis, Raman, Thermodynamics, Threonine genetics, Heme chemistry, Hemoglobins chemistry, Histidine chemistry, Peroxidases chemistry, Polychaeta chemistry, Threonine chemistry

Abstract

The activation of dehaloperoxidase-hemoglobin (DHP) to form a ferryl intermediate requires the distal histidine, H55, to act as an acid base catalyst. The lack of ancillary amino acids in the distal pocket to assist in this process makes H55 even more important to the formation of active intermediates than in conventional peroxidases. Therefore, one can infer that the precise conformation H55 may greatly affect the enzymatic activity. Using site-direct mutagenesis at position T56, immediately adjacent to H55, we have confirmed that subtle changes in the conformation of H55 affect the catalytic efficiency of DHP. Mutating T56 to a smaller amino acid appears to permit H55 to rotate with relatively low barriers between conformations in the distal pocket, which may lead to an increase in catalytic activity. On the other hand, larger amino acids in the neighboring site appear to restrict the rotation of H55 due to the steric hindrance. In the case of T56V, which is an isosteric mutation, H55 appears less mobile, but forced to be closer to the heme iron than in wild type. Both proximity to the heme iron and flexibility of motion in some of the mutants can result in an increased catalytic rate, but can also lead to protein inactivation due to ligation of H55 to the heme iron, which is known as hemichrome formation. A balance of enzymatic rate and protein stability with respect to hemichrome formation appears to be optimum in wild type DHP (WT-DHP)., (Copyright © 2013 Elsevier B.V. All rights reserved.)

Published

2013

40. Antithrombotic effects of a newly purified fibrinolytic protease from Urechis unicinctus.

Author

Bi Q, Han B, Feng Y, Jiang Z, Yang Y, and Liu W

Subjects

Animals, Chromatography, Ion Exchange, Female, Fibrinolytic Agents isolation & purification, Helminth Proteins chemistry, Helminth Proteins isolation & purification, Helminth Proteins pharmacology, Male, Mice, Peptide Hydrolases isolation & purification, Polychaeta chemistry, Rabbits, Rats, Rats, Wistar, Fibrinolytic Agents chemistry, Fibrinolytic Agents pharmacology, Peptide Hydrolases chemistry, Peptide Hydrolases pharmacology, Polychaeta enzymology, Thrombosis drug therapy

Abstract

Introduction: The prevalence of thromboembolic disease, one of the top 3 leading causes of mortality worldwide, is being reported continually. More effective and safer antithrombotic drugs may overcome the underlying problems in antithrombotic therapy. In the present work, antithrombotic effects of UFEIII, a newly purified fibrinolytic protease from Urechis unicinctus were evaluated., Materials and Methods: UFEIII was purified from the marine invertebrate, Urechis unicinctus, using anion exchange and gel filtration chromatography. Molecular weight, fibrinolytic activity and fibrinogenolysis pattern of UFEIII were determined. Furthermore, antithrombotic effects of UFEIII in vivo were investigated through electrical induced carotid arterial thrombosis in rats, FeCl3 induced carotid arterial thrombus model in rabbits and stasis induced vena caval thrombus model in rats., Results: SDS-PAGE of the purified enzyme showed a single polypeptide chain with molecular weight of 20.8kDa. In fibrin plate assays, UFEIII could not only directly degrade fibrin but also activate plasminogen. The fibrinogenolysis pattern of UFEIII was Aα-chains>Bβ-chains>γ-chain. Moreover, UFEIII could effectively prolong the time to occlusion in electrical induced carotid arterial thrombosis. Besides, both in rabbits and rats, the administration of UFEIII not only prolonged the activated partial thromboplastin time (APTT) and thrombin time (TT) also decreased the fibrinogen (FIB) content. Further, the thrombus lysis was observed after administration of UFEIII both in rabbits and rats., Conclusion: UFEIII can possibly be a new potential source of fibrinolytic agent., (© 2013 Elsevier Ltd. All rights reserved.)

Published

2013

41. UFEIII, a fibrinolytic protease from the marine invertebrate, Urechis unicinctus.

Author

Bi Q, Han B, Liu W, Feng Y, and Jiang Z

Subjects

Animals, Chromatography, Liquid, Electrophoresis, Polyacrylamide Gel, Enzyme Stability, Fibrinolytic Agents chemistry, Helminth Proteins chemistry, Hydrogen-Ion Concentration, Kinetics, Molecular Weight, Serine Proteases chemistry, Temperature, Fibrinolytic Agents isolation & purification, Helminth Proteins isolation & purification, Polychaeta enzymology, Serine Proteases isolation & purification

Abstract

A new serine protease with fibrinolytic activity from a marine invertebrate, Urechis unicinctus, was purified to electrophoretic homogeneity using column chromatography. SDS-PAGE of the purified enzyme showed a single polypeptide chain with MW ~20.8 kDa. Its N-terminal sequence was IIGGSQAAITSY. The purified enzyme, UFEIII, was stable at pH 6-10 below 60 °C with an optimum pH of 8.5 at approx. 55 °C. The enzyme activity was significantly inhibited by PMSF and SBTI suggesting that it was a serine protease. In fibrin plate assays, UFEIII was contained 1.46 × 10(3 )U (urokinase units) mg(-1) total fibrinolytic activity, which consisted of 692 U mg(-1) direct fibrinolytic activity and 769 U mg(-1) plasminogen-activator activity. Km and Vmax values for azocasein were 1 mg ml(-1) and 43 μg min(-1) ml(-1), respectively.

Published

2013

42. Three novel cytochrome P450 genes identified in the marine polychaete Perinereis nuntia and their transcriptional response to xenobiotics.

Author

Zheng S, Chen B, Qiu X, Lin K, and Yu X

Subjects

Amino Acid Sequence, Animals, Base Sequence, China, Cloning, Molecular, Conserved Sequence genetics, DNA Primers genetics, DNA, Complementary genetics, Gas Chromatography-Mass Spectrometry, Molecular Sequence Data, Polychaeta classification, Polychaeta genetics, Polycyclic Aromatic Hydrocarbons analysis, Polycyclic Aromatic Hydrocarbons toxicity, Reverse Transcriptase Polymerase Chain Reaction, Sequence Analysis, DNA, Sequence Homology, Species Specificity, Cytochrome P-450 Enzyme System genetics, Cytochrome P-450 Enzyme System metabolism, Environmental Monitoring methods, Gene Expression Regulation, Enzymologic drug effects, Polychaeta enzymology, Water Pollutants, Chemical toxicity, Xenobiotics toxicity

Abstract

Polychaetes have previously been used as bioindicators of environmental pollution. Their ability to eliminate organic pollutants such as polycyclic aromatic hydrocarbons (PAH) has been extensively analyzed. However, the cytochrome P450 monooxygenases (CYP) genes in polychaetes, which catalyze the first step of oxidative degradation of PAHs, have received little attention. Based on the partial sequences of three CYP genes that were enriched by subtractive cDNA libraries of the polychaete Perinereis nuntia, we amplified and sequenced the full-length cDNA of these novel CYP genes. These genes were named CYP4BB2, CYP423A1 and CYP424A1 by the Cytochrome P450 Nomenclature Committee. The deduced amino acid sequence of CYP4BB2 in P. nuntia showed 68% sequence identity to CYP4BB1 in Nereis virens, and was listed as a new member of the CYP4BB subfamily. The sequence of CYP423A1 and CYP424A1 both share less than 40% sequence identity to all known CYP enzymes and were classed into new CYP families. CYP family members are composite parts of a larger group called a clan. CYP4BB2 and CYP424A1 are listed as CYP4 clan members, while CYP423A1 is of the CYP2 clan. The 3D structures of these P. nuntia CYPs were successfully predicted by homology-modeling using the SWISS-MODEL workspace. The models of CYP424A1 and CYP4BB2 were created using 1jpzB (CYP102A) as a template, while CYP423A1 utilized 3czhB (CYP2R1) as its template. The presence of characteristic CYP superfamily motifs, such as the F-G⋯C-G amino acid sequence, and the conservation of the three-dimensional CYP structure shown by the modeling, suggested that these novel P. nuntia CYP genes may contain conserved functional domains of CYP monooxygenases. To examine the effect of xenobiotics on living organisms, we analyzed the transcriptional levels of these three new CYP genes in sandworms (P. nuntia) exposed to seawater artificially contaminated with benzo[a]pyrene (BaP). We also exposed individuals to industrial wastewater collected from Quanzhou Bay, Fujian, China, which was known to be contaminated with PAHs. Worms exposed to BaP had significantly higher levels of CYP4BB2, CYP423A1 and CYP424A1 mRNA. Transcription was up-regulated 5.9-, 5.3- and 12.3-folds respectively compared with the control worms living in clean seawater. The transcriptional levels of CYPs in worms cultured in the diluted wastewater collected from Quanzhou Bay, all positively correlated with the levels of PAHs detected in the water. The transcriptional up-regulation of the three CYP genes observed in this study, suggest the monooxygenases encoded by these CYP genes may play an important role in the detoxification of PAHs in this polychaete worm. These CYPs maybe essential for the adaptation of worms to contaminated environments and may be useful in the assessment of xenobiotic exposure., (Copyright © 2013 Elsevier B.V. All rights reserved.)

Published

2013

43. Purification and characterization of a new serine protease with fibrinolytic activity from the marine invertebrate, Urechis unicinctus.

Author

Bi Q, Chu J, Feng Y, Jiang Z, Han B, and Liu W

Subjects

Amino Acid Sequence, Animals, Fibrinolytic Agents pharmacology, Helminth Proteins pharmacology, Hydrogen-Ion Concentration, Kinetics, Metals pharmacology, Mice, Molecular Sequence Data, Polychaeta enzymology, Sequence Homology, Amino Acid, Serine Proteases pharmacology, Temperature, Fibrinolytic Agents isolation & purification, Helminth Proteins isolation & purification, Serine Proteases isolation & purification

Abstract

A non-hemorrhagic, chymotrypsin-like serine protease, UFEII, was purified from the marine echiuroid worm, Urechis unicinctus, after a combination of chromatography steps. UFEII was monomeric, with an apparent molecular weight of 26.7 kDa via SDS-PAGE. The isoelectric point of UFEII was 4.03, and the maximum activity of the enzyme was observed at 50 °C and pH8.0. According to fibrin plate assays, UFEII could not only directly degrade fibrin and fibrinogen but also activate plasminogen. Further, UFEII preferentially hydrolyzed the fibrinogen γ-chain, followed by the Bβ-chains and Aα-chains. Moreover, ufeII, full length of the gene encoding UFEII, was obtained by RT-PCR, degenerated PCR, and nested PCR. The ufeII was determined to be a 906-bp cDNA containing an open reading frame of 795 bp encoding a putative protein of 264 amino acids with a predicted molecular weight of 27.03 kDa. Besides, UFEII exhibited no hemorrhagic effect. Overall, U. unicinctus may represent a potential source of new therapeutic agents in thrombolytic therapy.

Published

2013

44. Multipart copolyelectrolyte adhesive of the sandcastle worm, Phragmatopoma californica (Fewkes): catechol oxidase catalyzed curing through peptidyl-DOPA.

Author

Wang CS and Stewart RJ

Subjects

Animals, Biocatalysis, Catechol Oxidase isolation & purification, Cross-Linking Reagents isolation & purification, Electrolytes, Polychaeta chemistry, Adhesives chemistry, Catechol Oxidase chemistry, Cross-Linking Reagents chemistry, Levodopa analogs & derivatives, Levodopa chemistry, Polychaeta enzymology

Abstract

Tube-building sabellariid polychaetes have major impacts on the geology and ecology of shorelines worldwide. Sandcastle worms, Phragmatopoma californica (Fewkes), live along the western coast of North America. Individual sabellariid worms build tubular shells by gluing together mineral particles with a multipart polyelectrolytic adhesive. Distinct sets of oppositely charged components are packaged and stored in concentrated granules in separate cell types. Homogeneous granules contain sulfated macromolecules as counter-polyanion to polycationic Pc2 and Pc5 proteins, which become major components of the fully cured glue. Heterogeneous granules contain polyphosphoproteins, Pc3A/B, paired with divalent cations and polycationic Pc1 and Pc4 proteins. Both types of granules contain catechol oxidase that catalyzes oxidative cross-linking of L-DOPA. Co-secretion of catechol oxidase guarantees rapid and spatially homogeneous curing with limited mixing of the preassembled adhesive packets. Catechol oxidase remains active long after the glue is fully cured, perhaps providing an active cue for conspecific larval settlement.

Published

2013

45. Detection and characterisation of mutations responsible for allele-specific protein thermostabilities at the Mn-superoxide dismutase gene in the deep-sea hydrothermal vent polychaete Alvinella pompejana.

Author

Bruneaux M, Mary J, Verheye M, Lecompte O, Poch O, Jollivet D, and Tanguy A

Subjects

Amino Acid Sequence, Animals, Escherichia coli genetics, Gene Library, Half-Life, Hot Temperature, Hydrothermal Vents, Models, Molecular, Molecular Sequence Data, Oceans and Seas, Polychaeta enzymology, Reactive Oxygen Species metabolism, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Sequence Analysis, DNA, Superoxide Dismutase chemistry, Superoxide Dismutase metabolism, Superoxide Dismutase-1, Alleles, Mutation, Polychaeta genetics, Superoxide Dismutase genetics

Abstract

Alvinella pompejana (Polychaeta, Alvinellidae) is one of the most thermotolerant marine eukaryotes known to date. It inhabits chimney walls of deep-sea hydrothermal vents along the East Pacific Rise (EPR) and is exposed to various challenging conditions (e.g. high temperature, hypoxia and the presence of sulphides, heavy metals and radiations), which increase the production of dangerous reactive oxygen species (ROS). Two different allelic forms of a manganese-superoxide dismutase involved in ROS detoxification, ApMnSOD1 and ApMnSOD2, and differing only by two substitutions (M110L and A138G) were identified in an A. pompejana cDNA library. RFLP screening of 60 individuals from different localities along the EPR showed that ApMnSOD2 was rare (2 %) and only found in the heterozygous state. Dynamic light scattering measurements and residual enzymatic activity experiments showed that the most frequent form (ApMnSOD1) was the most resistant to temperature. Their half-lives were similarly long at 65 °C (>110 min) but exhibited a twofold difference at 80 °C (20.8 vs 9.8 min). Those properties are likely to be explained by the occurrence of an additional sulphur-containing hydrogen bond involving the M110 residue and the effect of the A138 residue on the backbone entropy. Our results confirm the thermophily of A. pompejana and suggest that this locus is a good model to study how the extreme thermal heterogeneity of the vent conditions may help to maintain old rare variants in those populations.

Published

2013

46. Structural and kinetic study of an internal substrate binding site in dehaloperoxidase-hemoglobin A from Amphitrite ornata.

Author

Zhao J, de Serrano V, Zhao J, Le P, and Franzen S

Subjects

2-Propanol chemistry, Animals, Crystallography, X-Ray, Dimethyl Sulfoxide chemistry, Hemoglobins metabolism, Kinetics, Methanol chemistry, Models, Molecular, Peroxidases metabolism, Phenols chemistry, Polychaeta chemistry, Polychaeta metabolism, Protein Conformation, Hemoglobins chemistry, Peroxidases chemistry, Polychaeta enzymology

Abstract

X-ray crystal structures of dehaloperoxidase-hemoglobin A (DHP A) from Amphitrite ornata soaked with substrate, 2,4,6-tribromophenol (2,4,6-TBP), in buffer solvent with added methanol (MeOH), 2-propanol (2-PrOH), and dimethyl sulfoxide (DMSO) reveal an internal substrate binding site deep in the distal pocket above the α-edge of the heme that is distinct from the previously determined internal inhibitor binding site. The peroxidase function of DHP A has most often been studied using 2,4,6-trichlorophenol (2,4,6-TCP) as a substrate analogue because of the low solubility of 2,4,6-TBP in an aqueous buffer solution. Previous studies at low substrate concentrations pointed to the binding of substrate 2,4,6-TCP at an external site near the exterior heme β- or δ-edge as observed in the class of heme peroxidases. Here we report that the turnover frequencies of both substrates 2,4,6-TCP and 2,4,6-TBP deviate from Michaelis-Menten kinetics at high concentrations. The turnover frequency reaches a maximum in the range of 1400-1700 μM, with a decrease in rate at higher concentrations that is both substrate- and solvent-dependent. The X-ray crystal structure is consistent with the presence of an internal active site above the heme α-edge, in which the substrate would be oxidized in two consecutive steps inside the enzyme, followed by attack by H2O via a water channel in the protein. The physiological role of the internal site may involve interactions with any of a number of aromatic toxins found in benthic ecosystems where A. ornata resides.

Published

2013

47. Role of polarity of the distal pocket in the control of inhibitor binding in dehaloperoxidase-hemoglobin.

Author

Plummer A, Thompson MK, and Franzen S

Subjects

Animals, Binding Sites, Crystallography, X-Ray, Hemoglobins antagonists & inhibitors, Hemoglobins genetics, Models, Molecular, Peroxidases antagonists & inhibitors, Peroxidases genetics, Phenols metabolism, Point Mutation, Polychaeta chemistry, Polychaeta genetics, Polychaeta metabolism, Protein Binding, Substrate Specificity, Hemoglobins chemistry, Hemoglobins metabolism, Peroxidases chemistry, Peroxidases metabolism, Polychaeta enzymology

Abstract

Dehaloperoxidase (DHP A), a unique multifunctional enzyme, from the marine annelid Amphitrite ornata dehalogenates 2,4,6-tribromophenol to form 2,6-dibromo-1,4-benzoquinone. The catalytic cycle of DHP is similar to that of horseradish peroxidase (HRP), involving a high-valent ferryl heme and two single-electron transfers from the aromatic substrate to the enzyme. Like HRP, DHP has been investigated as a potential bioremediation enzyme. However, DHP fails as a bioremediation enzyme because, unlike HRP, it has an internal binding cavity on the distal side of the heme capable of accommodating p-bromophenols, which act as an inhibitor of peroxidase function. Blocking internal binding in DHP may be the key to allowing the enzyme to function effectively as a peroxidase on the full range of halogenated phenols. The distal cavity of DHP is surrounded by several hydrophobic amino acids that stabilize internal binding of the monohalogenated phenols, including a leucine residue near the back edge of the heme (L100). We have expressed the L100F, L100Q, L100T, and L100V mutants of DHP in an effort to prevent internal binding and thereby convert the inhibitors into substrates. Kinetic assays and resonance Raman indicate that the peroxidase activity of the L100T and L100F mutants is increased compared to that of native DHP in the presence of 4-bromophenol (4-BP), suggesting a reduction in the inhibitor binding constant. In addition, the X-ray crystal structure of L100F clearly indicates a reduced occupancy of the 4-BP inhibitor in the distal cavity of DHP. However, at the same time, the L100F structure reveals that steric interference alone is insufficient to exclude the inhibitor. Instead, the comparison of L100T and isosteric L100V reveals that an increase in polarity plays a decisive role in excluding the inhibitor from the distal binding pocket.

Published

2013

48. Catalytic efficiency of dehaloperoxidase A is controlled by electrostatics--application of the vibrational Stark effect to understand enzyme kinetics.

Author

Schkolnik G, Utesch T, Zhao J, Jiang S, Thompson MK, Mroginski MA, Hildebrandt P, and Franzen S

Subjects

Animals, Catalysis, Kinetics, Mutation, Peroxidase genetics, Peroxidases genetics, Protein Conformation, Spectroscopy, Fourier Transform Infrared, Peroxidase chemistry, Peroxidases chemistry, Polychaeta enzymology, Static Electricity, Vibration

Abstract

The vibrational Stark effect is gaining popularity as a method for probing electric fields in proteins. In this work, we employ it to explain the effect of single charge mutations in dehaloperoxidase-hemoglobin A (DHP A) on the kinetics of the enzyme. In a previous communication published in this journal (BBRC 2012, 420, 733-737) it has been shown that an increase in the overall negative charge of DHP A through mutation causes a decrease in its catalytic efficiency. Here, by labeling the protein with 4-mercaptobenzonitrile (MBN), a Stark probe molecule, we provide further evidence that the diffusion control of the catalytic process arises from the electrostatic repulsion between the enzyme and the negatively charged substrate. The linear correlation observed between the nitrile stretching frequency of the protein-bound MBN and the catalytic efficiency of the single-site mutants of the enzyme indicates that electrostatic interactions play a dominant role in determining the catalytic efficiency of DHP A., (Copyright © 2012 Elsevier Inc. All rights reserved.)

Published

2013

49. Study of the electrostatic effects of mutations on the surface of dehaloperoxidase-hemoglobin A.

Author

Zhao J, Rowe J, Franzen J, He C, and Franzen S

Subjects

Animals, Hemoglobin A genetics, Mutagenesis, Mutation, Peroxidases genetics, Recombinant Proteins chemistry, Recombinant Proteins genetics, Hemoglobin A chemistry, Peroxidases chemistry, Polychaeta enzymology, Static Electricity

Abstract

Point mutations of dehaloperoxidase-hemoglobin A (DHP A) that affect the surface charge have been prepared to study the interaction between DHP A with its substrate 2,4,6-trichlorophenol (TCP). Kinetic studies of these surface mutations showed a correlation, in which the more positively charged mutants have increased catalytic efficiency compared with wild type DHP A. As a result, the hypothesis of this study is that there is a global electrostatic interaction between DHP A and TCP. The electrostatic nature of substrate binding was further confirmed by the result that kinetic assays of DHP A were affected by ionic strength. Furthermore, isoelectric focusing (IEF) gel study showed that the pI-6.8 for DHP A, which indicates that DHP A has a slight negative charge pH 7, consistent with the kinetic observations., (Copyright © 2012 Elsevier Inc. All rights reserved.)

Published

2012

50. Nonphotochemical base-catalyzed hydroxylation of 2,6-dichloroquinone by H2O2 occurs by a radical mechanism.

Author

Franzen S, Sasan K, Sturgeon BE, Lyon BJ, Battenburg BJ, Gracz H, Dumariah R, and Ghiladi R

Subjects

Animals, Benzoquinones chemistry, Catalysis, Chlorophenols metabolism, Polychaeta metabolism, Benzoquinones metabolism, Hydrogen Peroxide metabolism, Peroxidases metabolism, Polychaeta enzymology

Abstract

Kinetic and structural studies have shown that peroxidases are capable of the oxidation of 2,4,6-trichlorophenol (2,4,6-TCP) to 2,6-dichloro-1,4-benzoquinone (2,6-DCQ). Further reactions of 2,6-DCQ in the presence of H(2)O(2) and OH(-) yield 2,6-dichloro-3-hydroxy-1,4-benzoquinone (2,6-DCQOH). The reactions of 2,6-DCQ have been monitored spectroscopically [UV-visible and electron spin resonance (ESR)] and chromatographically. The hydroxylation product, 2,6-DCQOH, has been observed by UV-visible and characterized structurally by (1)H and (13)C NMR spectroscopy. The results are consistent with a nonphotochemical base-catalyzed oxidation of 2,6-DCQ at pH > 7. Because H(2)O(2) is present in peroxidase reaction mixtures, there is also a potential role for the hydrogen peroxide anion (HOO(-)). However, in agreement with previous work, we observe that the nonphotochemical epoxidation by H(2)O(2) at pH < 7 is immeasurably slow. Both room-temperature ESR and rapid-freeze-quench ESR methods were used to establish that the dominant nonphotochemical mechanism involves formation of a semiquinone radical (base -catalyzed pathway), rather than epoxidation (direct attack by H(2)O(2) at low pH). Analysis of the kinetics using an Arrhenius model permits determination of the activation energy of hydroxylation (E(a) = 36 kJ/mol), which is significantly lower than the activation energy of the peroxidase-catalyzed oxidation of 2,4,6-TCP (E(a) = 56 kJ/mol). However, the reaction is second order in both 2,6-DCQ and OH(-) so that its rate becomes significant above 25 °C due to the increased rate of formation of 2,6-DCQ that feeds the second-order process. The peroxidase used in this study is the dehaloperoxidase-hemoglobin (DHP A) from Amphitrite ornata , which is used to study the effect of a catalyst on the reactions. The control experiments and precedents in studies of other peroxidases lead to the conclusion that hydroxylation will be observed following any process that leads to the formation of the 2,6-DCQ at pH > 7, regardless of the catalyst used in the 2,4,6-TCP oxidation reaction., (© 2011 American Chemical Society)

Published

2012