Your search keyword '"Catalase isolation & purification"' showing total 377 results

1. Single-Step Purification of Catalase Enzyme From Human Blood Erythrocytes Using Affinity Chromatography Technique.

Author

Çıkrıkcı K and Gencer N

Subjects

Humans, Hydrogen-Ion Concentration, Temperature, Enzyme Stability, Kinetics, Hydrogen Peroxide chemistry, Spectroscopy, Fourier Transform Infrared methods, Molecular Weight, Catalase chemistry, Catalase isolation & purification, Catalase metabolism, Erythrocytes enzymology, Chromatography, Affinity methods

Abstract

In this study, we aimed to isolate and purify catalase from human blood erythrocytes by using a newly synthesized affinity gel. The synthesized ω -amino hexyl agarose-1,2,3-triazole-5-carboxylic acid affinity gel was analyzed by FT-IR. Then, different buffer, pH, and ionic strength parameters were optimized to determine the equilibration, washing, and elution buffer conditions. The catalase was purified from human blood erythrocytes with a specific activity of 45.58 EU/mg, purification fold of 529.50, and a yield of 0.416% using the synthesized new affinity gel. The purity and molecular weight of the enzyme were analyzed by SDS-PAGE, and a single band at 60 kDa was observed for catalase. The optimum reaction temperature of the catalase was found to be 30°C, while the thermal stability temperature was 60°C. The Km and Vmax of the enzyme for hydrogen peroxide were calculated at 0.125 mM and 2500 U mL -1 , respectively., Competing Interests: The authors declare no conflicts of interest., (Copyright © 2024 Kübra Çıkrıkcı and Nahit Gencer.)

Published

2024

2. Rapid and Simple Detection of Isoniazid-Resistant Mycobacterium tuberculosis Utilizing a DNA Chromatography-Based Technique.

Author

Kodera T, Yamaguchi T, Fukushima Y, Kobayashi K, Takarada Y, Chizimu JY, Nakajima C, Solo ES, Lungu PS, Kawase M, and Suzuki Y

Subjects

Antitubercular Agents pharmacology, DNA, Bacterial, Humans, Isoniazid pharmacology, Mycobacterium tuberculosis drug effects, Sensitivity and Specificity, Sequence Analysis, Tuberculosis, Multidrug-Resistant genetics, Bacterial Proteins isolation & purification, Catalase isolation & purification, Chromatography methods, Isoniazid isolation & purification, Mycobacterium tuberculosis genetics, Mycobacterium tuberculosis isolation & purification, Tuberculosis, Multidrug-Resistant diagnosis

Abstract

Despite the availability of anti-tuberculosis drugs, the treatment of tuberculosis has been complicated by drug-resistant tuberculosis. The early detection of drug resistance makes early treatment possible. However, the available tools are mainly for rifampicin resistance detection, and the existing isoniazid resistance detection method is expensive, highly technical, and complicated, making it unsustainable for use in developing nations. This study aimed to develop a simple, rapid, and low-cost diagnostic kit for isoniazid-resistant tuberculosis using the single-stranded tag hybridization method to target an isoniazid resistance-conferring mutation. Specificity and sensitivity were assessed using DNA extracted from 49 isoniazid-resistant and 41 isoniazid-susceptible Mycobacterium tuberculosis clinical isolates cultured in mycobacterial growth indicator tubes. Positive signals were observed on mutant and wild-type lines with 100% sensitivity and specificity compared with Sanger sequencing results. In contrast, no positive signal was observed for non-tuberculosis mycobacteria. The detection limit of this method was 10 3 CFU or less. The STH-PAS system for isoniazid-resistant M. tuberculosis detection developed in this study offers a better alternative to conventional phenotypic isoniazid resistance determination, which will be of both clinical and epidemiological significance in resource-limited nations.

Published

2021

3. Interaction of artemisinin protects the activity of antioxidant enzyme catalase: A biophysical study.

Author

Samal RR, Kumari K, Sahoo Y, Mishra SK, and Subudhi U

Subjects

Animals, Antioxidants metabolism, Artemisinins metabolism, Catalase isolation & purification, Catalase metabolism, Catalytic Domain, Cattle, Humans, Hydrogen Bonding, Liver chemistry, Liver enzymology, Molecular Docking Simulation, Protein Binding, Protein Conformation, alpha-Helical, Protein Conformation, beta-Strand, Protein Interaction Domains and Motifs, Protein Structure, Tertiary, Thermodynamics, Antioxidants chemistry, Artemisinins chemistry, Catalase chemistry

Abstract

The major antioxidant enzyme catalase is downregulated and the enzyme activity is compromised in various disease conditions such as malarial and cancer. Hence, the restoration and protection of catalase is a promising therapeutic strategy in disease management. In the present study, for the first time we have demonstrated the protective role of well-known anti-malarial drug Artemisinin (ART) on the time and temperature-induced degradation of bovine liver catalase (BLC) activity. The findings at different time intervals and at higher temperature showed the protective role of ART on BLC activity. Molecular docking studies suggested specific binding of ART on BLC through heme group interface which was further supported by cyclic voltammetry and dynamic light scattering study. The stabilization of BLC in presence of ART was mediated through forming a BLC-ART complex with reduced and shifted electrochemical peak and increased hydrodynamic diameter. ART substantially prevents the temperature-induced reduction in α-helical content with simultaneous increment in other secondary structures like antiparallel, parallel, β-turn and random coils. Nevertheless, the protective role of ART was accepted from the enhanced thermal stability and increased T m value of BLC in presence of ART at higher temperatures. Our results uncover the mechanism of interaction between ART with BLC and suggest the protective role of ART towards spatiotemporal alteration of BLC by preventing the structural and molecular change in BLC. Thus, the findings advocate ART as a potential therapeutic drug for diseases associated with reduced catalase activity., Competing Interests: Declaration of competing interest The authors declare no competing financial interests., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

4. Catalases of the polyextremophylic Andean isolate Acinetobacter sp. Ver 3 confer adaptive response to H 2 O 2 and UV radiation.

Author

Sartorio MG, Repizo GD, and Cortez N

Subjects

Antioxidants isolation & purification, Biocatalysis, Catalase genetics, Catalase isolation & purification, Acinetobacter enzymology, Antioxidants metabolism, Catalase metabolism, Hydrogen Peroxide pharmacology, Ultraviolet Rays

Abstract

The polyextremophilic strain Acinetobacter sp. Ver3 isolated from high-altitude Andean lakes exhibits elevated tolerance to UV-B radiation and to pro-oxidants, a feature that has been correlated to its unusually high catalase activity. The Ver3 genome sequence analysis revealed the presence of two genes coding for monofunctional catalases: AV3 KatE1 and AV3 KatE2, the latter harboring an N-terminal signal peptide. We show herein that AV3 KatE1 displays one of the highest catalytic activities reported so far and is constitutively expressed at relatively high amounts in the cytosol, acting as the main protecting catalase against H 2 O 2 and UV-B radiation. The second catalase, AV3 KatE2, is a periplasmic enzyme strongly induced by both peroxide and UV, conferring supplementary protection against pro-oxidants. The N-terminal signal present in AV3 KatE2 was required not only for transport to the periplasm via the twin-arginine translocation pathway, but also for proper folding and subsequent catalytic activity. The analysis of catalase distribution among 114 Acinetobacter complete genomes revealed a great variability in the catalase classes, with A. baumannii clinical isolates exhibiting higher numbers of isoenzymes and the most variable profiles., (© 2020 Federation of European Biochemical Societies.)

Published

2020

5. [Expression, purification and characterization of catalase from Corynebacterium glutamicum].

Author

Yang H, Zhang X, Ma Z, Xu N, and Liu J

Subjects

Enzyme Activation, Enzyme Stability, Hydrogen-Ion Concentration, Catalase genetics, Catalase isolation & purification, Catalase metabolism, Corynebacterium glutamicum enzymology, Gene Expression Regulation, Enzymologic

Abstract

Catalase catalyzes the decomposition of H₂O₂ to H₂O and O₂, and has a wide range of industrial applications. However, most catalases used in the textile and paper industries are often subjected to high-alkaline challenges which makes it necessary to develop alkaline catalase. In this study, a catalase from Corynebacterium glutamicum was expressed in Escherichia coli, and the expression conditions were optimized. The recombinant catalase was purified by Ni-chelating affinity chromatography, and the recombinant enzyme was characterized. The optimal conditions of producing the recombinant catalase were: an IPTG concentration of 0.2 mmol/L, a culturing temperature of 25 °C and a culturing time of 11 h. The purified catalase had a specific activity of 55 266 U/mg, and it had a high activity in the pH range of 4.0 to11.5, with the highest activity at pH 11.0. When treated in pH 11.0 for 3 h, the enzyme retained 93% of its activity, indicating that the enzyme was qualified with a favorable stability under high-alkaline condition. The recombinant catalase had maximal activity at 30 °C, and showed a satisfactory thermal stability at a range of 25 °C to 50 °C. The apparent Km and Vmax values of purified catalase were 25.89 mmol/L and 185.18 mmol/(minmg), respectively. Besides, different inhibitors, such as sodium dodecyl sulfate (SDS), urea, NaN₂, β-mercaptoethanol, and EDTA had different degrees of inhibition on enzyme activity. The catalase from C. glutamicum shows high catalytic efficiency and high alkaline stability, suggesting its potential utilization in industrial production.

Published

2020

6. Purification and characterization of Terfezia claveryi TcCAT-1, a desert truffle catalase upregulated in mycorrhizal symbiosis.

Author

Marqués-Gálvez JE, Morte A, Navarro-Ródenas A, García-Carmona F, and Pérez-Gilabert M

Subjects

Catalase isolation & purification, Cistaceae growth & development, Droughts, Gene Expression Regulation, Enzymologic, Hydrogen Peroxide chemistry, Mycelium enzymology, Phylogeny, Catalase chemistry, Cistaceae microbiology, Mycorrhizae enzymology, Symbiosis genetics

Abstract

Terfezia claveryi Chatin is a mycorrhizal fungus that forms ectendomycorrhizal associations with plants of Helianthemum genus. Its appreciated edibility and drought resistance make this fungus a potential alternative crop in arid and semiarid areas of the Mediterranean region. In order to increase the knowledge about the biology of this fungus in terms of mycorrhiza formation and response to drought stress, a catalase from T. claveryi (TcCAT-1) has been purified to apparent homogeneity and biochemically characterized; in addition, the expression pattern of this enzyme during different stages of T. claveryi biological cycle and under drought stress conditions are reported. The results obtained, together with the phylogenetic analysis and homology modeling, indicate that TcCAT-1 is a homotetramer large subunit size monofunctional-heme catalase belonging to Clade 2. The highest expression of this enzyme occurs in mature mycorrhiza, revealing a possible role in mycorrhiza colonization, but it is not upregulated under drought stress. However, the H2O2 content of mycorrhizal plants submitted to drought stress is lower than in well watered treatments, suggesting that mycorrhization improves the plant's oxidative stress response, although not via TcCAT-1 upregulation., Competing Interests: The authors have read the journal’s policy and the authors of this manuscript have the following competing interests: JEMG is a paid employee of Thader Biotechnology SL. AM and ANR are partners of Thader Biotechnology SL. Thader Biotechnology is a spin-off company from the research group led by AM at the University of Murcia. AM is the co-founder and R&D director of this research group. ANR is the Technical director of this research group. There are no patents, products in development or marketed products associated with this research to declare. This does not alter our adherence to PLOS ONE policies on sharing data and materials.

Published

2019

7. Rapid detection of drug-resistant Mycobacterium tuberculosis directly from clinical specimens using allele-specific polymerase chain reaction assay.

Author

Sinha P, Banerjee T, Srivastava GN, and Anupurba S

Subjects

Alleles, Antitubercular Agents therapeutic use, Bacterial Proteins genetics, Bacterial Proteins isolation & purification, Catalase genetics, Catalase isolation & purification, DNA-Directed RNA Polymerases genetics, DNA-Directed RNA Polymerases isolation & purification, Female, Humans, Isoniazid adverse effects, Isoniazid therapeutic use, Male, Mutation, Mycobacterium tuberculosis genetics, Mycobacterium tuberculosis pathogenicity, Oxidoreductases genetics, Oxidoreductases isolation & purification, Rifampin adverse effects, Rifampin therapeutic use, Sputum microbiology, Tuberculosis, Multidrug-Resistant genetics, Tuberculosis, Multidrug-Resistant microbiology, Drug Resistance, Multiple, Bacterial genetics, Multiplex Polymerase Chain Reaction, Mycobacterium tuberculosis isolation & purification, Tuberculosis, Multidrug-Resistant diagnosis

Abstract

Background & Objectives: Rapid detection of drug resistance in Mycobacterium tuberculosis (MTB) is essential for the efficient control of tuberculosis. Hence, in this study a nested-allele-specific (NAS) PCR, nested multiple allele-specific PCR (NMAS-PCR) and multiple allele-specific (MAS) PCR assays were evaluated that enabled detection of the most common mutations responsible for isoniazid (INH) and rifampicin (RIF) resistance in MTB isolates directly from clinical specimens., Methods: Six pairs of primers, mutated and wild type, were used for the six targets such as codon 516, 526 and 531 of rpoB, codon 315 of katG and C15-T substitution in the promoter region of mabA-inhA using allele-specific (AS) PCR assays (NAS-PCR, NMAS-PCR and MAS-PCR). The performance of AS PCR method was compared with phenotypic drug susceptibility testing (DST)., Results: The usefulness of AS PCR assays was evaluated with 391 clinical specimens (251 Acid fast bacilli smear positive and MTB culture positive; 93 smear negative and MTB culture positive; 47 smear positive and MTB culture negative) and 344 MTB culture positive isolates. With culture-based phenotypic DST as a reference standard, the sensitivity and specificity of the NAS-PCR, NMAS-PCR and MAS-PCR assay for drug resistance-related genetic mutation detection were 98.6 and 97.8 per cent for INH, 97.5 and 97.9 per cent for RIF and 98.9 and 100 per cent for multidrug resistance (MDR)., Interpretation & Conclusions: The performance of AS PCR assays showed that those could be less expensive and technically executable methods for rapid detection of MDR-TB directly from clinical specimens., Competing Interests: None

Published

2019

8. The Usefulness of Performing Biochemical Tests in the Saliva of Kickboxing Athletes in the Dynamic of Training.

Author

Volodchenko OA, Podrigalo LV, Iermakov SS, Żychowska MT, and Jagiełło W

Subjects

Adolescent, Adult, Athletic Performance, Catalase isolation & purification, Catalase metabolism, Fatigue pathology, Fatigue prevention & control, Glycolysis genetics, Humans, Lactic Acid isolation & purification, Lipid Peroxidation genetics, Male, Pyruvic Acid isolation & purification, Pyruvic Acid metabolism, Saliva metabolism, Young Adult, Athletes, Fatigue metabolism, Lactic Acid metabolism, Saliva chemistry

Abstract

The study aimed to determine the suitability of testing the saliva of kickboxing athletes to show changes in biochemical parameters in dynamic of training. 8 elite male athletes (mean age 17.29± 0.31 years, body mass 66.82± 3.46kg, with 5.62±0.96 years of training experience) participated in the study. Indicators of lipid peroxidation and glycolysis (the concentration of lactic acid and pyruvic acid) were defined before and after a training session. Significant increases in indicators of lipid peroxidation activity indicators and the concentration of lactic acid (4-fold) were observed; analysis of correlation matrices confirms the absence of expressed changes. At the same time, significant decreases in catalase (10-fold from 3.69 μ kat/L to 0.39 μ kat/L) and pyruvic acid (from 3.92 μ l/l to 0.55 μ l/l) were observed. Our results confirm the value of using saliva to determine training load in an individual. Moreover, the study provided information on the importance of indexes reflecting a correlation of various biochemical indicators to estimate the sufficiency of training loads. The ease of sampling and informational content of saliva are reasons to use such tests in monitoring athletes' functional state to prevent fatigue.

Published

2019

9. Partial characterization of Bacillus pumilus catalase partitioned in poly(ethylene glycol)/sodium sulfate aqueous two-phase systems.

Author

Yuzugullu Karakus Y and Isik S

Subjects

Catalase isolation & purification, Enzyme Stability, Hydrogen-Ion Concentration, Molecular Weight, Temperature, Water chemistry, Bacillus pumilus enzymology, Catalase chemistry, Polyethylene Glycols chemistry, Solid Phase Extraction methods, Sulfates chemistry

Abstract

Aqueous two-phase partitioning system (ATPS) was used to extract and purify catalase from Bacillus pumilus. The system parameters for effective purification of catalase were optimized. The best catalase recovery (123%) with a 4.6-fold purification was obtained in the bottom phase of ATPS including the mixture of 15% (w/w) PEG4000, 10% (w/w) Na 2 SO 4 and 3% (w/w) NaCl at pH 5.0. The purified enzyme was characterized regarding its activity and stability. The highest enzyme activity was observed at pH 7.0 and 37 °C on hydrogen peroxide. The enzyme was quite stable at temperatures between 30 and 55 °C and a pH range of 7.0-9.0. The K m and V max values were determined from Lineweaver-Burk plot as 11 mM and 1667 µmole ml -1  min -1 , respectively. Overall, it can be said that ATPS is a rapid, reasonable, straightforward and cost-effective process for catalase purification in comparison to the chromatographic methods.

Published

2019

10. The novel multi cross-linked enzyme aggregates of protease, lipase, and catalase production from the sunflower seeds, characterization and application.

Author

Özacar M, Mehde AA, Mehdi WA, Özacar ZZ, and Severgün O

Subjects

Ammonium Sulfate chemistry, Biocatalysis, Catalase isolation & purification, Coloring Agents isolation & purification, Cross-Linking Reagents chemistry, Detergents chemistry, Enzyme Assays, Glutaral chemistry, Helianthus enzymology, Kinetics, Lipase isolation & purification, Peptide Hydrolases isolation & purification, Plant Proteins isolation & purification, Protein Aggregates, Seeds enzymology, Serum Albumin, Bovine chemistry, Starch chemistry, Catalase chemistry, Helianthus chemistry, Lipase chemistry, Peptide Hydrolases chemistry, Plant Proteins chemistry, Seeds chemistry

Abstract

The cross-linked enzyme aggregates (CLEAs) have numerous economic advantages in the industrial bio catalysis. In the present study, the multi CLEAs containing protease, catalase, and lipase from the sunflower seeds using starch as a cofeeder as well as bovine serum albumin (BSA) are designed and prepared successfully. After optimization, multi CLEAs of enzyme have been prepared with ammonium sulfate (55% w/v), glutaraldehyde (100 mM), and 8 mg/mL of starch or 20 mg/mL of BSA. The activity recovery of protease, catalase, and lipase multi CLEAs-starch are 87, 61, and 60%, respectively. Whereas, CLEAs prepared with BSA are 74, 61, and 50% activity and multi CLEAs only 60, 44, and 41% of protease, catalase, and lipase, respectively. The multi CLEAs were used to catalyze the reactions for enhanced washing process. After adding multi CLEAs-starch, the stain removal percentage of detergents is enhanced by 83%.The present study reports a high stability, simplicity, low cost, and recyclability of the novel multi CLEAs from the sunflower seeds that make them efficient as a highly active biocatalysts in the biotechnological applications. We believe that these novel multi CLEAs present a new approach to the synthesis of multi enzyme biocatalysts from the cheap and friendly environmental sources., (Copyright © 2018 Elsevier B.V. All rights reserved.)

Published

2019

11. Immobilization of Recombinant Human Catalase on Gold and Silver Nanoparticles.

Author

Pudlarz AM, Czechowska E, Ranoszek-Soliwoda K, Tomaszewska E, Celichowski G, Grobelny J, and Szemraj J

Subjects

Blotting, Western, Catalase isolation & purification, Electrophoresis, Polyacrylamide Gel, Enzymes, Immobilized genetics, Enzymes, Immobilized isolation & purification, Escherichia coli genetics, Humans, Light, Microscopy, Electron, Scanning Transmission, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Scattering, Radiation, Solutions, Surface Properties, Water, Catalase metabolism, Enzymes, Immobilized metabolism, Gold chemistry, Metal Nanoparticles chemistry, Silver chemistry

Abstract

Human catalase cDNA was cloned into a pEX-C-His vector. Purified recombinant catalase was immobilized on nanoparticles. Gold and silver nanoparticles were synthesized in a variety of sizes by chemical reduction; no agglomerates or aggregates were observed in any of the colloids during dynamic light scattering or scanning transmission electron microscopy analysis. After immobilization on gold nanoparticles, recombinant catalase activity was found to be lower than that of the same amount of enzyme in aqueous solution. However, after 10 days of storage at room temperature, the activity of catalase immobilized on gold nanoparticles (AuNPs) of 13 and 20 nm and coverage of 133% was 68 and 83% greater than catalase in aqueous solution, respectively. During 10 days of experiment, percentage activity of catalase immobilized on those gold nanoparticles was higher in comparison to CAT in aqueous solution. Catalase immobilized on silver nanoparticles did not lose activity as significantly as catalase immobilized on AuNPs. Those results confirm the ability to produce recombinant human enzymes in a bacterial expression system and its potential use while immobilized on silver or gold nanoparticles.

Published

2018

12. Comparison of Experimental and Broken Symmetry Density Functional Theory Calculated Electron Paramagnetic Resonance Parameters for the Manganese Catalase Active Site in the Superoxidized Mn III /Mn IV State.

Author

Beal NJ, Corry TA, and O'Malley PJ

Subjects

Binding Sites, Catalase chemistry, Catalase isolation & purification, Lactobacillus plantarum enzymology, Manganese chemistry, Models, Molecular, Superoxides chemistry, Thermus thermophilus enzymology, Catalase metabolism, Electron Spin Resonance Spectroscopy, Manganese metabolism, Quantum Theory, Superoxides metabolism

Abstract

Broken symmetry density functional theory has been used to calculate g-tensor, 55 Mn, 14 N, and 17 O hyperfine couplings for active site models of superoxidized Mn III /Mn IV manganese catalase both in its native and azide-inhibited form. While a good agreement is found between the calculated and experimental g-tensor and 55 Mn hyperfine couplings for all models, the active site geometry and Mn ion oxidation state can only be readily distinguished based on a comparison of the calculated and experimental 14 N azide and 17 O HFCs. This comparison shows that only models containing a Jahn-Teller distorted 5-coordinate (Mn III ) 2 site and a 6-coordinate (Mn IV ) 1 site can satisfactorily reproduce the experimental 14 N and 17 O hyperfine couplings.

Published

2018

13. Employment of proteomic and immunological based methods for the identification of catalase as novel allergen from banana.

Author

Nikolić J, Nešić A, Kull S, Schocker F, Jappe U, and Gavrović-Jankulović M

Subjects

Allergens analysis, Catalase analysis, Food Hypersensitivity diagnosis, Fruit enzymology, Fruit immunology, Humans, Immunoglobulin E immunology, Musa enzymology, Plant Proteins analysis, Plant Proteins immunology, Blotting, Western methods, Catalase isolation & purification, Food Hypersensitivity etiology, Musa immunology, Proteomics methods

Abstract

Diagnostic reagents based on food allergen extracts often lack sufficient sensitivity. The introduction of well characterized food allergens in molecular allergy diagnosis has been recognized as valid approach to circumvent unstandardized allergen extracts. Banana fruit (Musa acuminata) is a well-established allergen source which besides six characterized allergens, contains unidentified IgE reactive proteins whose clinical relevance remains undefined. By employment of a combinatorial peptide ligand library (CPLL) methodology with 2-D PAGE, mass spectrometric and 2-D immunoblot analysis, a novel allergen from banana fruit was detected in banana as catalase. A recombinant homologue of natural catalase was produced, isolated and biochemically characterized. The recombinant protein showed IgE reactivity in 7 out of 13 tested patients with suspected allergy to banana in immunoblot. Novel banana fruit allergens should be added as components to allergen-microarrays for the diagnosis and the monitoring of banana allergy., Significance: By employment of CPLL methodology with 2-D PAGE, mass spectrometric and 2-D immunoblot analysis catalase from banana fruit is identified as a novel allergen, with proposed designation as Mus a 7. IgE reactive recombinant Mus a 7 was produced and should be included in a component-resolved allergy diagnosis., (Copyright © 2018 Elsevier B.V. All rights reserved.)

Published

2018

14. Purification of camel liver catalase by zinc chelate affinity chromatography and pH gradient elution: An enzyme with interesting properties.

Author

Chafik A, Essamadi A, Çelik SY, and Mavi A

Subjects

Animals, Camelus, Catalase antagonists & inhibitors, Catalase metabolism, Edetic Acid, Enzyme Inhibitors, Hydrogen-Ion Concentration, Sodium Dodecyl Sulfate, Temperature, Catalase chemistry, Catalase isolation & purification, Chromatography, Affinity methods, Liver enzymology

Abstract

Climate change and increasing temperatures are global concerns. Camel (Camelus dromedarius) lives most of its life under high environmental stress in the desert and represent ideal model for studying desert adaptation among mammals. Catalase plays a key role in protecting cells against oxidative stress. For the first time, catalase from camel liver was purified to homogeneity by zinc chelate affinity chromatography using pH gradient elution, a better separation was obtained. A purification fold of 201.81 with 1.17% yield and a high specific activity of 1132539.37U/mg were obtained. The native enzyme had a molecular weight of 268kDa and was composed of four subunits of equal size (65kDa). The enzyme showed optimal activity at a temperature of 45°C and pH 7.2. Thiol reagents, β-Mercaptoethanol and D,L-Dithiothreitol, inhibited the enzyme activity. The enzyme was inhibited by Al 3+ , Cd 2+ and Mg 2+ , whereas Ca 2+ , Co 2+ and Ni 2+ stimulated the catalase activity. Reduced glutathione has no effect on catalase activity. The K m and V max of the enzyme for hydrogen peroxide were 37.31mM and 6185157U/mg, respectively. Sodium azide inhibited the enzyme noncompetitively with K i value of 14.43μM, the IC 50 was found to be 16.71μM. The properties of camel catalase were different comparing to those of mammalian species. Relatively higher molecular weight, higher optimum temperature, protection of reduced glutathione from hydrogen peroxide oxidation and higher affinity for hydrogen peroxide and sodium azide, these could be explained by the fact that camel is able to live in the intense environmental stress in the desert., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2017

15. High production, purification, biochemical characterization and gene analysis of a novel catalase from the thermophilic bacterium Ureibacillus thermosphaericus FZSF03.

Author

Jia X, Lin X, Tian Y, Chen J, and You M

Subjects

Amino Acid Sequence, Bacillales drug effects, Bacillales genetics, Bacillales physiology, Carbon pharmacology, Catalase isolation & purification, Catalase metabolism, Cloning, Molecular, Dose-Response Relationship, Drug, Fermentation drug effects, Hydrogen-Ion Concentration, Kinetics, Nitrogen pharmacology, Bacillales enzymology, Catalase biosynthesis, Catalase genetics, Temperature

Abstract

A catalase-producing thermophilic bacterium, Ureibacillus thermosphaericus FZSF03, was isolated from high-temperature compost. Catalase production in this strain increased 31 times and reached 57,630U/mL after optimization in a shake flask, which might represent the highest catalase activity level among reported wild strains. This catalase was further purified and identified. The purified enzyme showed a specific activity of 219,360U/mg, higher than many other catalases. The molecular weight of this enzyme is 52kDa according to sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE), and the enzyme was identified as a monofunctional haeme catalase of Ureibacillus thermosphaericus by liquid chromatography-mass spectrometry (LC-MS)/MS. The optimal reaction temperature for this catalase was found to be 60°C. Stability was observed at 60°C and at a pH of 10.0, indicating the superiority of this enzyme at a high temperature and under alkaline conditions. Therefore, this catalase is a prospective candidate for industrial production and applications. The gene encoding this catalase is 1503bp. As the amino acid sequence shows low similarity with other catalases, we suggest that this is a novel monofunctional haeme catalase., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2017

16. Elucidating the interaction of clofazimine with bovine liver catalase; a comprehensive spectroscopic and molecular docking approach.

Author

Zaman M, Nusrat S, Zakariya SM, Khan MV, Ajmal MR, and Khan RH

Subjects

Animals, Binding Sites, Catalase isolation & purification, Cattle, Crystallography, X-Ray, Hydrogen Bonding, Hydrophobic and Hydrophilic Interactions, Liver enzymology, Protein Binding, Protein Conformation, alpha-Helical, Protein Conformation, beta-Strand, Protein Interaction Domains and Motifs, Spectrum Analysis methods, Thermodynamics, Catalase chemistry, Clofazimine chemistry, Liver chemistry, Molecular Docking Simulation

Abstract

Nowadays, understanding of interface between protein and drugs has become an active research area of interest. These types of interactions provide structural guidelines in drug design with greater clinical efficacy. Thus, structural changes in catalase induced by clofazimine were monitored by various biophysical techniques including UV-visible spectrometer, fluorescence spectroscopy, circular dichroism, and dynamic light scattering techniques. Increase in absorption spectra (UV-visible spectrum) confers the complex formation between drug and protein. Fluorescence quenching with a binding constants of 2.47 × 10 4  M -1 revealed that clofazimine binds with protein. Using fluorescence resonance energy transfer, the distance (r) between the protein (donor) and drug (acceptor) was found to be 2.89 nm. Negative Gibbs free energy change (ΔG°) revealed that binding process is spontaneous. In addition, an increase in α-helicity was observed by far-UV circular dichroism spectra by adding clofazimine to protein. Dynamic light scattering results indicate that topology of bovine liver catalase was slightly altered in the presence of clofazimine. Hydrophobic interactions are the main forces between clofazimine and catalase interaction as depicted by molecular docking studies. Apart from hydrophobic interactions, some hydrogen bonding was also observed during docking method. The results obtained from the present study may establish abundant in optimizing the properties of ligand-protein mixtures relevant for numerous formulations., (Copyright © 2017 John Wiley & Sons, Ltd.)

Published

2017

17. Electrochemical monitoring of native catalase activity in skin using skin covered oxygen electrode.

Author

Nocchi S, Björklund S, Svensson B, Engblom J, and Ruzgas T

Subjects

Antioxidants metabolism, Catalase chemistry, Catalysis, Electrodes, Epidermis chemistry, Humans, Hydrogen Peroxide chemistry, Hydrogen-Ion Concentration, Oxygen metabolism, Biosensing Techniques, Catalase isolation & purification, Epidermis enzymology, Skin enzymology

Abstract

A skin covered oxygen electrode, SCOE, was constructed with the aim to study the enzyme catalase, which is part of the biological antioxidative system present in skin. The electrode was exposed to different concentrations of H 2 O 2 and the amperometric current response was recorded. The observed current is due to H 2 O 2 penetration through the outermost skin barrier (referred to as the stratum corneum, SC) and subsequent catalytic generation of O 2 by catalase present in the underlying viable epidermis and dermis. By tape-stripping the outermost skin layers we demonstrate that SC is a considerable diffusion barrier for H 2 O 2 penetration. Our experiments also indicate that skin contains a substantial amount of catalase, which is sufficient to detoxify H 2 O 2 that reaches the viable epidermis after exposure of skin to high concentrations of peroxide (0.5-1mM H 2 O 2 ). Further, we demonstrate that the catalase activity is reduced at acidic pH, as compared with the activity at pH 7.4. Finally, experiments with often used penetration enhancer thymol shows that this compound interferes with the catalase reaction. Health aspect of this is briefly discussed. Summarizing, the results of this work show that the SCOE can be utilized to study a broad spectrum of issues involving the function of skin catalase in particular, and the native biological antioxidative system in skin in general., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2017

18. [Proteomic analysis of contaminants in recombinant membrane hemeproteins expressed in E. coli and isolated by metal affinity chromatography].

Author

Yantsevich AV, Dzichenka YV, Ivanchik AV, Shapiro MA, Trawkina M, Shkel TV, Gilep AA, Sergeev GV, and Usanov SA

Subjects

Amino Acid Sequence, Catalase isolation & purification, Cloning, Molecular, Escherichia coli genetics, Escherichia coli metabolism, Flavoproteins genetics, Flavoproteins metabolism, Gene Expression, Genetic Vectors chemistry, Genetic Vectors metabolism, Glutamine-Fructose-6-Phosphate Transaminase (Isomerizing) isolation & purification, Heat-Shock Proteins isolation & purification, Hemeproteins genetics, Hemeproteins metabolism, Humans, Peptide Elongation Factor Tu isolation & purification, Peptidylprolyl Isomerase isolation & purification, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Ribosomal Proteins isolation & purification, Sepharose analogs & derivatives, Sepharose chemistry, Chromatography, Affinity methods, Escherichia coli Proteins isolation & purification, Flavoproteins isolation & purification, Hemeproteins isolation & purification, Proteomics methods

Abstract

Contaminating proteins have been identified by “shotgun” proteomic analysis in 14 recombinant preparations of human membrane heme- and flavoproteins expressed in Escherichia coli and purified by immobilized metal ion affinity chromatography. Immobilized metal ion affinity chromatography of ten proteins was performed on Ni2+-NTA-sepharose 6B, and the remaining four proteins were purified by ligand affinity chromatography on 2',5'-ADP-sepharose 4B. Proteomic analysis allowed to detect 50 protein impurities from E. coli. The most common contaminant was Elongation factor Tu2. It is characterized by a large dipole moment and a cluster arrangement of acidic amino acid residues that mediate the specific interaction with the sorbent. Peptidyl prolyl-cis-trans isomerase SlyD, glutamine-fructose-6-phosphate aminotransferase, and catalase HPII that contained repeating HxH, QxQ, and RxR fragments capable of specific interaction with the sorbent were identified among the protein contaminants as well. GroL/GroS chaperonins were probably copurified due to the formation of complexes with the target proteins. The Ni2+ cations leakage from the sorbent during lead to formation of free carboxyl groups that is the reason of cation exchanger properties of the sorbent. This was the putative reason for the copurification of basic proteins, such as the ribosomal proteins of E. coli and the widely occurring uncharacterized protein YqjD. The results of the analysis revealed variation in the contaminant composition related to the type of protein expressed. This is probably related to the reaction of E. coli cell proteome to the expression of a foreign protein. We concluded that the nature of the protein contaminants in a preparation of a recombinant protein purified by immobilized metal ion affinity chromatography on a certain sorbent could be predicted if information on the host cell proteome were available.

Published

2017

19. Isolation and Abiotic Stress Resistance Analyses of a Catalase Gene from Ipomoea batatas (L.) Lam.

Author

Yong B, Wang X, Xu P, Zheng H, Fei X, Hong Z, Ma Q, Miao Y, Yuan X, Jiang Y, and Shao H

Subjects

Gene Expression Regulation, Enzymologic physiology, Gene Expression Regulation, Plant physiology, Open Reading Frames, Plant Leaves enzymology, Plant Leaves genetics, Plant Tubers enzymology, Plant Tubers genetics, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Sequence Analysis, DNA, Catalase chemistry, Catalase genetics, Catalase isolation & purification, Catalase metabolism, Ipomoea batatas enzymology, Ipomoea batatas genetics, Plant Proteins genetics, Plant Proteins isolation & purification, Plant Proteins metabolism, Stress, Physiological

Abstract

As an indicator of the antioxidant capability of plants, catalase can detoxify reactive oxygen species (ROS) generated by environmental stresses. Sweet potato is one of the top six most important crops in the world. However, its catalases remain largely unknown. In this study, a catalase encoding gene, IbCAT2 (accession number: KY615708), was identified and cloned from sweet potato cv. Xushu 18. It contained a 1479 nucleotides' open reading frame (ORF). S-R-L, Q-K-L, and a putative calmodulin binding domain were located at the C-terminus of IbCAT2, which suggests that IbCAT2 could be a peroxisomal catalase. Next-generation sequencing (NGS) based quantitative analyses showed that IbCAT2 was mainly expressed in young leaves and expanding tuberous roots under normal conditions. When exposed to 10% PEG6000 or 200 mmol/L NaCl solutions, IbCAT2 was upregulated rapidly in the first 11 days and then downregulated, although different tissues showed different degree of change. Overexpression of IbCAT2 conferred salt and drought tolerance in Escherichia coli and Saccharomyces cerevisiae . The positive response of IbCAT2 to abiotic stresses suggested that IbCAT2 might play an important role in stress responses.

Published

2017

20. Biochemical characterization of a catalase from Vibrio vulnificus, a pathogen that causes gastroenteritis.

Author

Pei J, Wang H, Wu L, Xia S, Xu C, Zheng B, Li T, and Jiang Y

Subjects

Catalase isolation & purification, Chromatography, Affinity, Cloning, Molecular, Computer Simulation, Enzyme Stability, Gene Expression Regulation, Bacterial, Heme metabolism, Hydrogen-Ion Concentration, Mutagenesis, Site-Directed, Phylogeny, Protein Engineering methods, Recombinant Proteins genetics, Temperature, Vibrio vulnificus physiology, Catalase genetics, Catalase metabolism, Vibrio vulnificus enzymology

Abstract

Vibrio vulnificus is a virulent human pathogen causing gastroenteritis and possibly life threatening septicemia in patients. Most V. vulnificus are catalase positive and can deactivate peroxides, thus allowing them to survive within the host. In the study presented here, a catalase from V. vulnificus (CAT-Vv) was purified to homogeneity after expression in Escherichia coli. The kinetics and function of CAT-Vv were examined. CAT-Vv catalyzed the reduction of H 2 O 2 at an optimal pH of 7.5 and temperature of 35°C. The V max and K m values were 65.8±1.2 U/mg and 10.5±0.7 mM for H 2 O 2 , respectively. Mutational analysis suggests that amino acids involved in heme binding play a key role in the catalysis. Quantitative reverse transcription-PCR revealed that in V. vulnificus, transcription of CAT-Vv was upregulated by low salinity, heat, and oxidative stresses. This research gives new clues to help inhibit the growth of, and infection by V. vulnificus.

Published

2017

21. Isolation and polyphasic characterization of a novel hyper catalase producing thermophilic bacterium for the degradation of hydrogen peroxide.

Author

Sooch BS, Kauldhar BS, and Puri M

Subjects

Geobacillus genetics, Hydrogen-Ion Concentration, RNA, Bacterial genetics, RNA, Ribosomal, 16S genetics, Bacterial Proteins biosynthesis, Bacterial Proteins chemistry, Bacterial Proteins isolation & purification, Catalase biosynthesis, Catalase chemistry, Catalase isolation & purification, Geobacillus enzymology, Hydrogen Peroxide chemistry

Abstract

A newly isolated microbial strain of thermophilic genus Geobacillus has been described with emphasis on polyphasic characterization and its application for degradation of hydrogen peroxide. The validation of this thermophilic strain of genus Geobacillus designated as BSS-7 has been demonstrated by polyphasic taxonomy approaches through its morphological, biochemical, fatty acid methyl ester profile and 16S rDNA sequencing. This thermophilic species of Geobacillus exhibited growth at broad pH and temperature ranges coupled with production of extraordinarily high quantities of intracellular catalase, the latter of which as yet not been reported in any member of this genus. The isolated thermophilic bacterial culture BSS-7 exhibited resistance against a variety of organic solvents. The immobilized whole cells of the bacterium successfully demonstrated the degradation of hydrogen peroxide (H2O2) in a packed bed reactor. This strain has potential application in various analytical and diagnostic methods in the form of biosensors and biomarkers in addition to applications in the textile, paper, food and pharmaceutical industries.

Published

2016

22. Comparative study of enzymatic activities of new KatG mutants from low- and high-level isoniazid-resistant clinical isolates of Mycobacterium tuberculosis.

Author

Brossier F, Boudinet M, Jarlier V, Petrella S, and Sougakoff W

Subjects

Bacterial Proteins isolation & purification, Bacterial Proteins metabolism, Catalase isolation & purification, Catalase metabolism, Drug Resistance, Bacterial genetics, Humans, Microbial Sensitivity Tests methods, Models, Molecular, Mutation, Mycobacterium tuberculosis drug effects, Mycobacterium tuberculosis enzymology, Mycobacterium tuberculosis isolation & purification, Tuberculosis drug therapy, Antitubercular Agents pharmacology, Bacterial Proteins genetics, Catalase genetics, Isoniazid pharmacology, Mycobacterium tuberculosis genetics, Tuberculosis microbiology

Abstract

Resistance to isoniazid (INH-R) in Mycobacterium tuberculosis is mainly due to mutations at position 315 (S315T) of the catalase-peroxidase KatG. We identified 16 mutations (including 13 biochemically uncharacterized mutations) in KatG from INH-R clinical isolates of M. tuberculosis showing mutations other than S315T. The KatG enzymatic activities (catalase, peroxidase, free radical production and isonicotinoyl-NAD formation) of wild-type KatG and the 16 mutants were determined and correlated to their spatial location in a KatG model structure. Of all mutations studied, H270R, which conferred a high level of INH-R and results in the disruption of a coordination bond with the heme, caused complete loss of all enzymatic KatG activities. The mutants generally associated with a very high level of INH-R were all characterized by a drastic reduction in catalase activity and a marked decrease in INH activation activities. One mutant, A162E, displayed a behavior similar to S315T, i.e. a moderate decrease in catalase activity and a drastic decrease in the formation of the radical form of INH. Finally, the mutants associated with a low level of INH-R showed a moderate reduction in the four catalytic activities, likely stemming from an overall alteration of the folding and/or stability of the KatG protein., (Copyright © 2016 Elsevier Ltd. All rights reserved.)

Published

2016

23. Catalase purification from rat liver with iron-chelated poly(hydroxyethyl methacrylate-N-methacryloyl-(l)-glutamic acid) cryogel discs.

Author

Göktürk I, Perçin I, and Denizli A

Subjects

Adsorption, Animals, Catalase chemistry, Glutamic Acid chemistry, Hydrogen-Ion Concentration, Microscopy, Electron, Scanning, Osmolar Concentration, Rats, Temperature, Catalase isolation & purification, Cryogels, Glutamic Acid analogs & derivatives, Iron Chelating Agents chemistry, Liver enzymology, Methacrylates chemistry

Abstract

In this study, iron-chelated poly(hydroxyethyl methacrylate-N-methacryloyl-(l)-glutamic acid) (PHEMAGA/Fe(3+)) cryogel discs were prepared. The PHEMAGA/Fe(3+) cryogel discs were characterized by elemental analysis, scanning electron microscopy, Fourier transform infrared spectroscopy, swelling tests, and surface area measurements. The PHEMAGA/Fe(3+) cryogel discs had large pores ranging from 10 to 100 µm with a swelling degree of 9.36 g H2O/g cryogel. Effects of pH, temperature, initial catalase concentration, and flow rate on adsorption capacity of the PHEMAGA/Fe(3+) cryogel discs were investigated. Maximum catalase adsorption capacity (62.6 mg/g) was obtained at pH 7.0, 25°C, and 3 mg/ml initial catalase concentration. The PHEMAGA/Fe(3+) cryogel discs were also tested for the purification of catalase from rat liver. After tissue homogenization, purification of catalase was performed using the PHEMAGA/Fe(3+) cryogel discs and catalase was obtained with a yield of 54.34 and 16.67 purification fold.

Published

2016

24. Engineering of a novel tri-functional enzyme with MnSOD, catalase and cell-permeable activities.

Author

Luangwattananun P, Yainoy S, Eiamphungporn W, Songtawee N, Bülow L, Ayudhya CI, and Prachayasittikul V

Subjects

Catalase chemistry, Catalase genetics, Catalase isolation & purification, Cell Line, Chromatography, Gel, Enzyme Activation, Heme chemistry, Humans, Models, Molecular, Molecular Weight, Oxidation-Reduction, Oxidative Stress, Protein Conformation, Recombinant Fusion Proteins, Superoxide Dismutase chemistry, Superoxide Dismutase genetics, Superoxide Dismutase isolation & purification, Catalase metabolism, Cell Membrane Permeability, Protein Engineering, Superoxide Dismutase metabolism

Abstract

Cooperative function of superoxide dismutase (SOD) and catalase (CAT), in protection against oxidative stress, is known to be more effective than the action of either single enzyme. Chemical conjugation of the two enzymes resulted in molecules with higher antioxidant activity and therapeutic efficacy. However, chemical methods holds several drawbacks; e.g., loss of enzymatic activity, low homogeneity, time-consuming, and the need of chemical residues removal. Yet, the conjugated enzymes have never been proven to internalize into target cells. In this study, by employing genetic and protein engineering technologies, we reported designing and production of a bi-functional protein with SOD and CAT activities for the first time. To enable cellular internalization, cell penetrating peptide from HIV-1 Tat (TAT) was incorporated. Co-expression of CAT-MnSOD and MnSOD-TAT fusion genes allowed simultaneous self-assembly of the protein sequences into a large protein complex, which is expected to contained one tetrameric structure of CAT, four tetrameric structures of MnSOD and twelve units of TAT. The protein showed cellular internalization and superior protection against paraquat-induced cell death as compared to either complex bi-functional protein without TAT or to native enzymes fused with TAT. This study not only provided an alternative strategy to produce multifunctional protein complex, but also gained an insight into the development of therapeutic agent against oxidative stress-related conditions., (Copyright © 2016 Elsevier B.V. All rights reserved.)

Published

2016

25. Microbial communities affecting albumen photography heritage: a methodological survey.

Author

Puškárová A, Bučková M, Habalová B, Kraková L, Maková A, and Pangallo D

Subjects

Adsorption, Bacteria classification, Bacteria enzymology, Bacteria genetics, Bacterial Proteins metabolism, Bacterial Typing Techniques, Biodegradation, Environmental, Catalase isolation & purification, Catalase metabolism, Collodion chemistry, DNA, Intergenic genetics, Fungal Proteins metabolism, Fungi classification, Fungi enzymology, Fungi genetics, History, 19th Century, History, 20th Century, Humans, Lipase isolation & purification, Lipase metabolism, Microbial Consortia physiology, Mycological Typing Techniques, Peroxidase isolation & purification, Peroxidase metabolism, Photography methods, RNA, Ribosomal, 16S genetics, Salts chemistry, Spectrometry, X-Ray Emission, Spectroscopy, Fourier Transform Infrared, Albumins chemistry, Bacteria isolation & purification, Bacterial Proteins isolation & purification, Fungal Proteins isolation & purification, Fungi isolation & purification, Photography history

Abstract

This study is one of the few investigations which analyze albumen prints, perhaps the most important photographic heritage of the late 19(th) and early 20(th) centuries. The chemical composition of photographic samples was assessed using Fourier-transform infrared spectroscopy and X-ray fluorescence. These two non-invasive techniques revealed the complex nature of albumen prints, which are composed of a mixture of proteins, cellulose and salts. Microbial sampling was performed using cellulose nitrate membranes which also permitted the trapped microflora to be observed with a scanning electron microscope. Microbial analysis was performed using the combination of culture-dependent (cultivation in different media, including one 3% NaCl) and culture-independent (bacterial and fungal cloning and sequencing) approaches. The isolated microorganisms were screened for their lipolytic, proteolytic, cellulolytic, catalase and peroxidase activities. The combination of the culture-dependent and -independent techniques together with enzymatic assays revealed a substantial microbial diversity with several deteriogen microorganisms from the genera Bacillus, Kocuria, Streptomyces and Geobacillus and the fungal strains Acrostalagmus luteoalbus, Bjerkandera adusta, Pleurotus pulmonarius and Trichothecium roseum.

Published

2016

26. Color reduction of melanin by lysosomal and peroxisomal enzymes isolated from mammalian cells.

Author

Park DJ, Sekhon SS, Yoon J, Kim YH, and Min J

Subjects

Catalase metabolism, Enzyme Activation, HeLa Cells, Humans, Lysosomes physiology, Muramidase metabolism, Oxidative Stress, Peroxisomes physiology, Reactive Oxygen Species metabolism, Ultraviolet Rays, Catalase isolation & purification, Lysosomes enzymology, Melanins metabolism, Muramidase isolation & purification, Peroxisomes enzymology

Abstract

Lysosomes and peroxisomes are organelles with many functions in all eukaryotic cells. Lysosomes contain hydrolytic enzymes (lysozyme) that degrade molecules, whereas peroxisomes contain enzymes such as catalase that convert hydrogen peroxide (H2O2) to water and oxygen and neutralize toxicity. In contrast, melanin is known as a helpful element to protect the skin against harmful ultraviolet rays. However, a high quantity of melanin leads to hyperpigmentation or skin cancer in human. New materials have already been discovered to inhibit tyrosinase in melanogenesis; however, melanin reduction does not suggest their preparation. In this study, we report that the color intensity because of melanin decreased by the cellular activation of lysosomes and peroxisomes. An increase in the superficial intensity of lysosome and peroxisome activities of HeLa cells was observed. In addition, a decrease in the amount of melanin has also been observed in mammalian cells without using any other chemical, showing that the process can work in vivo for treating melanin. Therefore, the results of this study indicate that the amount of melanin decreases by the lysosome and peroxisome activity after entering the cells, and functional organelles are effective in color reduction. This mechanism can be used in vivo for treating melanin.

Published

2016

27. Isolation of lactic acid bacteria exhibiting high scavenging activity for environmental hydrogen peroxide from fermented foods and its two scavenging enzymes for hydrogen peroxide.

Author

Watanabe A, Kaneko C, Hamada Y, Takeda K, Kimata S, Matsumoto T, Abe A, Tanaka N, Okada S, Uchino M, Satoh J, Nakagawa J, and Niimura Y

Subjects

Amino Acid Sequence, Catalase chemistry, Catalase isolation & purification, Catalase metabolism, Cloning, Molecular, Culture Media chemistry, Oryza microbiology, Oxidation-Reduction, Pediococcus pentosaceus enzymology, Pediococcus pentosaceus genetics, Peroxidases chemistry, Peroxidases isolation & purification, Peroxidases metabolism, Raphanus microbiology, Vegetables microbiology, Catalase genetics, Fermentation, Food Microbiology, Hydrogen Peroxide metabolism, Pediococcus pentosaceus isolation & purification, Pediococcus pentosaceus metabolism, Peroxidases genetics

Abstract

To obtain lactic acid bacteria that scavenge environmental hydrogen peroxide, we developed a specialized enrichment medium and successfully isolated Pediococcus pentosaceus Be1 strain from a fermented food. This strain showed vigorous environmental hydrogen peroxide scavenging activity over a wide range of hydrogen peroxide concentrations. High Mn-catalase and NADH peroxidase activities were found in the cell-free extract of the P. pentosaceus Be1 strain, and these two hydrogen peroxide scavenging enzymes were purified from the cell-free extract of the strain. Mn-catalase has been purified from several microorganisms by several researchers, and the NADH peroxidase was first purified from the original strain in this report. After cloning the genes of the Mn-catalase and the NADH peroxidase, the deduced amino acid sequences were compared with those of known related enzymes.

Published

2016

28. Cloning, Expression, and Characterization of a Novel Thermophilic Monofunctional Catalase from Geobacillus sp. CHB1.

Author

Jia X, Chen J, Lin C, and Lin X

Subjects

Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Bacterial Proteins biosynthesis, Bacterial Proteins chemistry, Bacterial Proteins genetics, Bacterial Proteins isolation & purification, Catalase biosynthesis, Catalase chemistry, Catalase genetics, Catalase isolation & purification, Cloning, Molecular, Gene Expression, Geobacillus enzymology, Geobacillus genetics

Abstract

Catalases are widely used in many scientific areas. A catalase gene (Kat) from Geobacillus sp. CHB1 encoding a monofunctional catalase was cloned and recombinant expressed in Escherichia coli (E. coli), which was the first time to clone and express this type of catalase of genus Geobacillus strains as far as we know. This Kat gene was 1,467 bp in length and encoded a catalase with 488 amino acid residuals, which is only 81% similar to the previously studied Bacillus sp. catalase in terms of amino acid sequence. Recombinant catalase was highly soluble in E. coli and made up 30% of the total E. coli protein. Fermentation broth of the recombinant E. coli showed a high catalase activity level up to 35,831 U/mL which was only lower than recombinant Bacillus sp. WSHDZ-01 among the reported catalase production strains. The purified recombinant catalase had a specific activity of 40,526 U/mg and K m of 51.1 mM. The optimal reaction temperature of this recombinant enzyme was 60°C to 70°C, and it exhibited high activity over a wide range of reaction temperatures, ranging from 10°C to 90°C. The enzyme retained 94.7% of its residual activity after incubation at 60°C for 1 hour. High yield and excellent thermophilic properties are valuable features for this catalase in industrial applications.

Published

2016

29. Novel immobilization process of a thermophilic catalase: efficient purification by heat treatment and subsequent immobilization at high temperature.

Author

Xu J, Luo H, López C, Xiao J, and Chang Y

Subjects

Enzyme Activation, Enzyme Stability, Bacillus enzymology, Catalase chemistry, Catalase isolation & purification, Enzymes, Immobilized chemistry, Enzymes, Immobilized isolation & purification, Heating methods

Abstract

The main goal of the present work is to investigate a novel process of purification and immobilization of a thermophilic catalase at high temperatures. The catalase, originated from Bacillus sp., was overexpressed in a recombinant Escherichia coli BL21(DE3)/pET28-CATHis and efficiently purified by heat treatment, achieving a threefold purification. The purified catalase was then immobilized onto an epoxy support at different temperatures (25, 40, and 55 °C). The immobilizate obtained at higher temperatures reached its maximum activity in a shorter time than that obtained at lower temperatures. Furthermore, immobilization at higher temperatures required a lower ionic strength than immobilization at lower temperatures. The characteristics of immobilized enzymes prepared at different temperatures were investigated. The high-temperature immobilizate (55 °C) showed the highest thermal stability, followed by the 40 °C immobilizate. And the high-temperature immobilizate (55 °C) had slightly higher operational stability than the 25 °C immobilizate. All of the immobilized catalase preparations showed higher stability than the free enzyme at alkaline pH 10.0, while the alkali resistance of the 25 °C immobilizate was slightly better than that of the 40 and 55 °C immobilizates.

Published

2015

30. A factor converting viable but nonculturable Vibrio cholerae to a culturable state in eukaryotic cells is a human catalase.

Author

Senoh M, Hamabata T, and Takeda Y

Subjects

Catalase isolation & purification, Cell Line, Chromatography, Liquid, Coculture Techniques, Electrophoresis, Polyacrylamide Gel, Humans, Tandem Mass Spectrometry, Vibrio cholerae O1 growth & development, Catalase metabolism, Eukaryotic Cells enzymology, Vibrio cholerae O1 physiology

Abstract

In our previous work, we demonstrated that viable but nonculturable (VBNC) Vibrio cholerae O1 and O139 were converted to culturable by coculture with eukaryotic cells. Furthermore, we isolated a factor converting VBNC V. cholerae to culturable (FCVC) from a eukaryotic cell line, HT-29. In this study, we purified FCVC by successive column chromatographies comprising UNO Q-6 anion exchange, Bio-Scale CHT2-1 hydroxyapatite, and Superdex 200 10/300 GL. Homogeneity of the purified FCVC was demonstrated by SDS-PAGE. Nano-LC MS/MS analysis showed that the purified FCVC was a human catalase. An experiment of RNAi knockdown of catalase mRNA from HT-29 cells and treatment of the purified FCVC with a catalase inhibitor, 3-amino-1,2,4-triazole confirmed that the FCVC was a catalase. A possible role of the catalase in converting a VBNC V. cholerae to a culturable state in the human intestine is discussed., (© 2015 The Authors. MicrobiologyOpen published by John Wiley & Sons Ltd.)

Published

2015

31. Propionibacterium acnes catalase induces increased Th1 immune response in sarcoidosis patients.

Author

Yorozu P, Furukawa A, Uchida K, Akashi T, Kakegawa T, Ogawa T, Minami J, Suzuki Y, Awano N, Furusawa H, Miyazaki Y, Inase N, and Eishi Y

Subjects

Adult, Aged, Animals, Catalase isolation & purification, Enzyme-Linked Immunosorbent Assay, Female, Humans, Male, Mice, Middle Aged, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Antigens, Bacterial immunology, Catalase immunology, Hypersensitivity immunology, Propionibacterium acnes enzymology, Propionibacterium acnes immunology, Sarcoidosis immunology, Th1 Cells immunology

Abstract

Background: Propionibacterium acnes is one of the most commonly implicated etiologic agents of sarcoidosis. We screened antigenic proteins from this indigenous bacterium that increase Th1 responses in sarcoidosis patients., Methods: Antigenic bacterial proteins were screened by probing western blots of P. acnes whole cell lysates with blood plasma samples from 52 sarcoidosis patients and 34 healthy volunteers. Soluble protein antigens from the bands most frequently detected on blotting membranes were analyzed by matrix-assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI-TOF/MS). Recombinant proteins were prepared from DNA sequences of the proteins identified by MALDI-TOF/MS and analyzed by immunologic assays., Results: MALDI-TOF/MS analysis identified propionyl-CoA carboxylase subunit beta, arginine deiminase (ADI), catalase (KAT), and UDP-N-acetylglucosamine pyrophosphorylase (UAP). Successfully prepared recombinant proteins from ADI, KAT, and UAP provoked humoral and cellular immune responses in mice immunized with P. acnes when measured by enzyme-linked immunosorbent assay for serum antibodies and enzyme-linked immunospot assay for interferon (IFN)-γ-secreting cells (ELISPOT IFN-γ assay) with lymph node cells. Plasma IgG and IgA titers to KAT and UAP were significantly higher in sarcoidosis patients than in healthy volunteers. When Th1 immune responses to ADI, KAT, and UAP were measured by ELISPOT IFN-γ assay with peripheral blood mononuclear cells from 12 sarcoidosis patients, 13 other pneumonitis patients, and 11 healthy volunteers, only the KAT protein provoked a significantly higher response in sarcoidosis patients (p=0.0032)., Conclusion: These results suggest that P. acnes KAT is an antigen that provokes allergic Th1 immune responses in sarcoidosis patients., (Copyright © 2015 The Japanese Respiratory Society. Published by Elsevier B.V. All rights reserved.)

Published

2015

32. Extraction of superoxide dismutase, catalase, and carbonic anhydrase from stroma-free red blood cell hemolysate for the preparation of the nanobiotechnological complex of polyhemoglobin-superoxide dismutase-catalase-carbonic anhydrase.

Author

Guo C, Gynn M, and Chang TM

Subjects

Animals, Biotechnology, Cattle, Hemolysis, Carbonic Anhydrases chemistry, Carbonic Anhydrases isolation & purification, Catalase chemistry, Catalase isolation & purification, Erythrocytes enzymology, Hemoglobins chemical synthesis, Hemoglobins chemistry, Superoxide Dismutase chemistry, Superoxide Dismutase isolation & purification

Abstract

We report a novel method to simultaneously extract superoxide dismutase (SOD), catalase (CAT), and carbonic anhydrase (CA) from the same sample of red blood cells (RBCs). This avoids the need to use expensive commercial enzymes, thus enabling a cost-effective process for large-scale production of a nanobiotechnological polyHb-SOD-CAT-CA complex, with enhancement of all three red blood cell functions. An optimal concentration of phosphate buffer for ethanol-chloroform treatment results in good recovery of CAT, SOD, and CA after extraction. Different concentrations of the enzymes can be used to enhance the activity of polyHb-SOD-CAT-CA to 2, 4, or 6 times that of RBC.

Published

2015

33. Reversible adsorption of catalase onto Fe(3+) chelated poly(AAm-GMA)-IDA cryogels.

Author

Aktaş Uygun D, Uygun M, Akgöl S, and Denizli A

Subjects

Adsorption, Animals, Cattle, Hydrogen-Ion Concentration, Kinetics, Microscopy, Electron, Scanning, Osmolar Concentration, Recycling, Spectrometry, X-Ray Emission, Spectroscopy, Fourier Transform Infrared, Temperature, Acrylic Resins chemistry, Catalase isolation & purification, Cryogels chemistry, Imino Acids chemistry, Iron Chelating Agents chemistry

Abstract

In this presented study, poly(acrylamide-glycidyl methacrylate) [poly(AAm-GMA)] cryogels were synthesized by cryopolymerization technique at sub-zero temperature. Prepared cryogels were then functionalized with iminodiacetic acid (IDA) and chelated with Fe(3+) ions in order produce the metal chelate affinity matrix. Synthesized cryogels were characterized with FTIR, ESEM and EDX analysis, and it was found that the cryogel had sponge like structure with interconnected pores and their pore diameter was about 200 μm. Fe(3+) chelated poly(AAm-GMA)-IDA cryogels were used for the adsorption of catalase and optimum adsorption conditions were determined by varying the medium pH, initial catalase concentration, temperature and ionic strength. Maximum catalase adsorption onto Fe(3+) chelated poly(AAm-GMA)-IDA cryogel was found to be 12.99 mg/g cryogel at 25 °C, by using pH 5.0 acetate buffer. Adsorbed catalase was removed from the cryogel by using 1.0M of NaCl solution and desorption yield was found to be 96%. Additionally, reusability profile of the Fe(3+) chelated poly(AAm-GMA)-IDA cryogel was also investigated and it was found that, adsorption capacity of the cryogels didn't decrease significantly at the end of the 40 reuses. Catalase activity studies were also tested and it was demonstrated that desorbed catalase retained 70% of its initial activity., (Copyright © 2015 Elsevier B.V. All rights reserved.)

Published

2015

34. Purification, biochemical characterization, and implications of an alkali-tolerant catalase from the spacecraft-associated and oxidation-resistant Acinetobacter gyllenbergii 2P01AA.

Author

Muster N, Derecho I, Dallal F, Alvarez R, McCoy KB, and Mogul R

Subjects

Amino Acid Sequence, Catalase antagonists & inhibitors, Catalase chemistry, Electrophoresis, Polyacrylamide Gel, Enzyme Stability drug effects, Hydrogen Peroxide pharmacology, Hydrogen-Ion Concentration, Kinetics, Mass Spectrometry, Models, Molecular, Molecular Sequence Data, Oxidation-Reduction drug effects, Sequence Homology, Amino Acid, Sodium Hydroxide pharmacology, Structural Homology, Protein, Temperature, Acinetobacter enzymology, Alkalies pharmacology, Catalase isolation & purification, Catalase metabolism, Spacecraft

Abstract

Herein, we report on the purification, characterization, and sequencing of catalase from Acinetobacter gyllenbergii 2P01AA, an extremely oxidation-resistant bacterium that was isolated from the Mars Phoenix spacecraft assembly facility. The Acinetobacter are dominant members of the microbial communities that inhabit spacecraft assembly facilities and consequently may serve as forward contaminants that could impact the integrity of future life-detection missions. Catalase was purified by using a 3-step chromatographic procedure, where mass spectrometry provided respective subunit and intact masses of 57.8 and 234.6 kDa, which were consistent with a small-subunit tetrameric catalase. Kinetics revealed an extreme pH stability with no loss in activity between pH 5 and 11.5 and provided respective kcat/Km and kcat values of ∼10(7) s(-1) M(-1) and 10(6) s(-1), which are among the highest reported for bacterial catalases. The amino acid sequence was deduced by in-depth peptide mapping, and structural homology suggested that the catalases from differing strains of A. gyllenbergii differ only at residues near the subunit interfaces, which may impact catalytic stability. Together, the kinetic, alkali-tolerant, and halotolerant properties of the catalase from A. gyllenbergii 2P01AA are significant, as they are consistent with molecular adaptations toward the alkaline, low-humidity, and potentially oxidizing conditions of spacecraft assembly facilities. Therefore, these results support the hypothesis that the selective pressures of the assembly facilities impact the microbial communities at the molecular level, which may have broad implications for future life-detection missions.

Published

2015

35. Purification, cloning, expression, and biochemical characterization of a monofunctional catalase, KatP, from Pigmentiphaga sp. DL-8.

Author

Dong W, Hou Y, Li S, Wang F, Zhou J, Li Z, Wang Y, Huang F, Fu L, Huang Y, and Cui Z

Subjects

Bacterial Proteins chemistry, Catalase chemistry, Bacterial Proteins isolation & purification, Burkholderiaceae enzymology, Catalase isolation & purification

Abstract

Catalases are essential components of the cellular equipment used to cope with oxidative stress. The monofunctional catalase KatP was purified from Pigmentiphaga sp. using ammonium sulfate precipitation (ASP), diethylaminoethyl ion exchange chromatography (IEC), and hydrophobic interaction chromatography (HIC). The purified catalase formed polymer with an estimated monomer molecular mass of 54kDa, which were resolved by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and zymogram analysis. KatP exhibited a specific catalytic activity of 73,000U/mg, which was higher than that of catalase-1 of Comamonas terrigena N3H (55,900U/mg). Seven short tryptic fragments of this catalase were obtained by electrospray ionization quadrupole time-of-flight mass spectrometry (ESI-Q-TOF MS/MS), and the gene, katP, was cloned by PCR amplification and overexpressed in Escherichia coli BL21 (DE3). Based on the complete amino acid sequence, KatP was identified as a clade 3 monofunctional catalase. The specific activities of recombinant KatP for hydrogen peroxide (690,000U/mg) increased 9-fold over that of the parent strain. The Km and Vmax of recombinant KatP were 9.48mM and 81.2mol/minmg, respectively. The optimal pH and temperature for KatP were 7.0 and 37°C, respectively, and the enzyme displayed abroad pH-stable range of 4.0-11.0. The enzyme was inhibited by Zn(2+), Cu(2+), Cr(2+), and Mn(2+), whereas Fe(3+) and Mg(2+) stimulated KatP enzymatic activity. Interestingly, the catalase activity of recombinant KatP displayed high stability under different temperature and pH conditions, suggesting that KatP is a potential candidate for the production of catalase., (Copyright © 2015 Elsevier Inc. All rights reserved.)

Published

2015

36. A simple method of catalase purification for the undergraduate experimental course.

Author

Chen Q, Cheng M, Wang Y, Yao M, Chen Y, Gao Y, and Ding W

Subjects

Animals, Blotting, Western, Catalase metabolism, Chromatography, Gel, Education, Medical, Undergraduate, Electrophoresis, Polyacrylamide Gel, Kinetics, Mice, Molecular Weight, Sulfates chemistry, Catalase isolation & purification

Abstract

Catalase is a characteristic enzyme of peroxisomes, of which it is the most abundant protein. This enzyme serves as a typical example of a peroxisomal enzyme and is important in the teaching of biochemistry and molecular biology. Although there is substantial information regarding catalase purification, purifying catalase for the junior‑grade undergraduate experimental course face challenges in obtaining materials and increasingly expensive purification equipment. This study presents a simple method for the purification of mouse liver catalase using ethanol‑chloroform treatment, sodium sulfate fractionation, dialysis and Sephadex G‑200 gel filtration chromatography. Catalase was purified 31.8‑fold with an 18.3% yield. The advantages of this method were its low operating environment requirements, simple procedure and reduced cost. Furthermore, the method was designed to improve students' comprehensive ability and manipulative ability and to introduce a sense of innovation in the fields of biochemistry and molecular biology during their junior year.

Published

2015

37. Purification and characterization of a mycelial catalase from Scedosporium boydii, a useful tool for specific antibody detection in patients with cystic fibrosis.

Author

Mina S, Marot-Leblond A, Cimon B, Fleury MJ, Larcher G, Bouchara JP, and Robert R

Subjects

Chromatography, Liquid methods, Enzyme-Linked Immunosorbent Assay methods, Humans, Molecular Weight, Mycelium enzymology, Protein Multimerization, Serologic Tests methods, Antibodies, Fungal blood, Antigens, Fungal chemistry, Antigens, Fungal isolation & purification, Catalase chemistry, Catalase isolation & purification, Cystic Fibrosis complications, Mycoses diagnosis, Scedosporium enzymology

Abstract

Scedosporium boydii is an opportunistic filamentous fungus which may be responsible for a wide variety of infections in immunocompetent and immunocompromised individuals. This fungus belongs to the Scedosporium apiospermum species complex, which usually ranks second among the filamentous fungi colonizing the airways of patients with cystic fibrosis (CF) and may lead to allergic bronchopulmonary mycoses, sensitization, or respiratory infections. Upon microbial infection, host phagocytic cells release reactive oxygen species (ROS), such as hydrogen peroxide, as part of the antimicrobial response. Catalases are known to protect pathogens against ROS by detoxification of the hydrogen peroxide. Here, we investigated the catalase equipment of Scedosporium boydii, one of the major pathogenic species in the S. apiospermum species complex. Three catalases were identified, and the mycelial catalase A1 was purified to homogeneity by a three-step chromatographic process. This enzyme is a monofunctional tetrameric protein of 460 kDa, consisting of four 82-kDa glycosylated subunits. The potential usefulness of this enzyme in serodiagnosis of S. apiospermum infections was then investigated by an enzyme-linked immunosorbent assay (ELISA), using 64 serum samples from CF patients. Whatever the species involved in the S. apiospermum complex, sera from infected patients were clearly differentiated from sera from patients with an Aspergillus fumigatus infection or those from CF patients without clinical and biological signs of a fungal infection and without any fungus recovered from sputum samples. These results suggest that catalase A1 is a good candidate for the development of an immunoassay for serodiagnosis of infections caused by the S. apiospermum complex in patients with CF., (Copyright © 2015, American Society for Microbiology. All Rights Reserved.)

Published

2015

38. Comparative analyses of universal extraction buffers for assay of stress related biochemical and physiological parameters.

Author

Han C, Chan Z, and Yang F

Subjects

Antioxidants chemistry, Ascorbate Peroxidases chemistry, Ascorbate Peroxidases isolation & purification, Buffers, Catalase chemistry, Catalase isolation & purification, Glutathione Reductase isolation & purification, Hydrogen Peroxide chemistry, Peroxidase chemistry, Peroxidase isolation & purification, Superoxide Dismutase chemistry, Superoxide Dismutase isolation & purification, Antioxidants isolation & purification, Glutathione Reductase chemistry, Oxidative Stress

Abstract

Comparative efficiency of three extraction solutions, including the universal sodium phosphate buffer (USPB), the Tris-HCl buffer (UTHB), and the specific buffers, were compared for assays of soluble protein, free proline, superoxide radical (O2∙-), hydrogen peroxide (H2O2), and the antioxidant enzymes such as superoxide dismutase (SOD), catalase (CAT), guaiacol peroxidase (POD), ascorbate peroxidase (APX), glutathione peroxidase (GPX), and glutathione reductase (GR) in Populus deltoide. Significant differences for protein extraction were detected via sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) and two-dimensional electrophoresis (2-DE). Between the two universal extraction buffers, the USPB showed higher efficiency for extraction of soluble protein, CAT, GR, O2∙-, GPX, SOD, and free proline, while the UTHB had higher efficiency for extraction of APX, POD, and H2O2. When compared with the specific buffers, the USPB showed higher extraction efficiency for measurement of soluble protein, CAT, GR, and O2∙-, parallel extraction efficiency for GPX, SOD, free proline, and H2O2, and lower extraction efficiency for APX and POD, whereas the UTHB had higher extraction efficiency for measurement of POD and H2O2. Further comparisons proved that 100 mM USPB buffer showed the highest extraction efficiencies. These results indicated that USPB would be suitable and efficient for extraction of soluble protein, CAT, GR, GPX, SOD, H2O2, O2∙-, and free proline.

Published

2015

39. Inhibitory effects of deferasirox on the structure and function of bovine liver catalase: a spectroscopic and theoretical study.

Author

Moradi M, Divsalar A, Saboury AA, Ghalandari B, and Harifi AR

Subjects

Animals, Binding, Competitive, Catalase chemistry, Catalase isolation & purification, Catalytic Domain, Cattle, Circular Dichroism, Deferasirox, Heme chemistry, Hydrophobic and Hydrophilic Interactions, Iron chemistry, Kinetics, Liver chemistry, Liver enzymology, Protein Binding, Protein Structure, Secondary, Solutions, Spectrometry, Fluorescence, Temperature, Thermodynamics, Tryptophan chemistry, Benzoates chemistry, Catalase antagonists & inhibitors, Enzyme Inhibitors chemistry, Iron Chelating Agents chemistry, Molecular Docking Simulation, Triazoles chemistry

Abstract

Deferasirox (DFX), as an oral chelator, is used for treatment of transfusional iron overload. In this study, we have investigated the effects of DFX as an iron chelator, on the function and structure of bovine liver catalase (BLC) by different spectroscopic methods of UV-visible, fluorescence, and circular dichroism (CD) at two temperatures of 25 and 37 °C. In vitro kinetic studies showed that DFX can inhibit the enzymatic activity in a competitive manner. KI value was calculated 39 nM according to the Lineweaver-Burk plot indicating a high rate of inhibition of the enzyme. Intrinsic fluorescence data showed that increasing the drug concentrations leads to a significant decrease in the intrinsic emission of the enzyme indicating a significant change in the three-dimensional environment around the chromophores of the enzyme structure. By analyzing the fluorescence quenching data, it was found that the BLC has two binding sites for DFX and the values of binding constant at 25 and 37 °C were calculated 1.7 × 10(7) and 3 × 10(7) M(-1), respectively. The static type of quenching mechanism is involved in the quenching of intrinsic emission of enzyme. The thermodynamic data suggest that hydrophobic interactions play a major role in the binding reaction. UV-vis spectroscopy results represented the changes in tryptophan (Trp) absorption and Soret band spectra, which indicated changes in Trp and heme group position caused by the drug binding. Also, CD data represented that high concentrations of DFX lead to a significant decreasing in the content of β-sheet and random coil accompanied an increasing in α-helical content of the protein. The molecular docking results indicate that docking may be an appropriate method for prediction and confirmation of experimental results and also useful for determining the binding mechanism of proteins and drugs. According to above results, it can be concluded that the DFX can chelate the Fe(III) on the enzyme active site leading to changes in the function and structure of catalase which can be considered as a side effect of this drug and consequently has an important role in hepatic complications and fibrosis.

Published

2015

40. Recent insights into microbial catalases: isolation, production and purification.

Author

Sooch BS, Kauldhar BS, and Puri M

Subjects

Bacterial Proteins chemistry, Bacterial Proteins genetics, Catalase chemistry, Catalase genetics, Fungal Proteins chemistry, Fungal Proteins genetics, Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Bacterial Proteins biosynthesis, Bacterial Proteins isolation & purification, Biotechnology methods, Catalase biosynthesis, Catalase isolation & purification, Fungal Proteins biosynthesis, Fungal Proteins isolation & purification

Abstract

Catalase, an oxidoreductase enzyme, works as a detoxification system inside living cells against reactive oxygen species formed as a by-product of different metabolic reactions. The enzyme is found in a wide range of aerobic and anaerobic organisms. Catalase has also been employed in various analytical and diagnostic methods in the form of biosensors and biomarkers in addition to its other applications in textile, paper, food and pharmaceutical industries. New applications for catalases are constantly emerging thanks to their high turnover rate, distinct evolutionary origin, relatively simple and well-defined reaction mechanisms. The following review provides comprehensive information on isolation, production and purification of catalases with different techniques from various microbial sources along with their types, structure, mechanism of action and applications., (Copyright © 2014 Elsevier Inc. All rights reserved.)

Published

2014

41. A bifunctional enzyme from Rhodococcus erythropolis exhibiting secondary alcohol dehydrogenase-catalase activities.

Author

Martinez-Rojas E, Kurt T, Schmidt U, Meyer V, and Garbe LA

Subjects

Alcohol Oxidoreductases chemistry, Alcohol Oxidoreductases isolation & purification, Catalase chemistry, Catalase isolation & purification, Cloning, Molecular, Coenzymes metabolism, Enzyme Stability, Escherichia coli genetics, Gene Expression, Lactones metabolism, Mass Spectrometry, NAD metabolism, Oxidation-Reduction, Rhodococcus genetics, Substrate Specificity, Temperature, Alcohol Oxidoreductases genetics, Alcohol Oxidoreductases metabolism, Catalase genetics, Catalase metabolism, Rhodococcus enzymology

Abstract

Alcohol dehydrogenases have long been recognized as potential biocatalyst for production of chiral fine and bulk chemicals. They are relevant for industry in enantiospecific production of chiral compounds. In this study, we identified and purified a nicotinamide adenine dinucleotide (NAD)-dependent secondary alcohol dehydrogenase (SdcA) from Rhodococcus erythropolis oxidizing γ-lactols into γ-lactones. SdcA showed broad substrate specificity on γ-lactols; secondary aliphatic alcohols with 8 and 10 carbon atoms were also substrates and oxidized with (2S)-stereospecificity. The enzyme exhibited moderate stability with a half-life of 5 h at 40 °C and 20 days at 4 °C. Mass spectrometric identification revealed high sequence coverage of SdcA amino acid sequence to a highly conserved catalase from R. erythropolis. The corresponding encoding gene was isolated from genomic DNA and subsequently overexpressed in Escherichia coli BL21 DE3 cells. In addition, the recombinant SdcA was purified and characterized in order to confirm that the secondary alcohol dehydrogenase and catalase activity correspond to the same enzyme.

Published

2014

42. In vitro and in vivo inhibitory effects of some fungicides on catalase produced and purified from white-rot fungus Phanerochaete chrysosporium.

Author

Kavakçıoğlu B and Tarhan L

Subjects

Anti-Bacterial Agents pharmacology, Catalase chemistry, Catalase isolation & purification, Culture Media chemistry, Culture Techniques, Enzyme Stability, Hydrogen-Ion Concentration, Kinetics, Phanerochaete growth & development, Phanerochaete metabolism, Temperature, Catalase antagonists & inhibitors, Catalase biosynthesis, Enzyme Inhibitors pharmacology, Fungicides, Industrial pharmacology, Phanerochaete enzymology

Abstract

In this study, in vitro and in vivo effects of some commonly used fungicides, antibiotics, and various chemicals on isolated and purified catalase from Phanerochaete chrysosporium were investigated. The catalase was purified 129.10-fold by using 60% ammonium sulfate and 60% ethanol precipitations, DEAE-cellulose anion exchange and Sephacryl-S-200 gel filtration chromatographies from P. chrysosporium growth in carbon- and nitrogen-limited medium for 12 days. The molecular weight of native purified catalase from P. chrysosporium was found to be 290 ± 10 kDa, and sodium dodecyl sulfate (SDS)-PAGE results indicated that enzyme consisted of four apparently identical subunits, with a molecular weight of 72.5 ± 2.5 kDa. Kinetic characterization studies showed that optimum pH and temperature, Km and Vmax values of the purified catalase which were stable in basic region and at comparatively high temperatures were 7.5, 30°C, 289.86 mM, and 250,000 U/mg, respectively. The activity of purified catalase from P. chrysosporium was significantly inhibited by dithiothreitol (DTT), 2-mercaptoethanol, iodoacetamide, EDTA, and sodium dodecyl sulfate (SDS). It was found that while antibiotics had no inhibitory effects, 45 ppm benomyl, 144 ppm captan, and 47.5 ppm chlorothalonil caused 14.52, 10.82, and 38.86% inhibition of purified catalase, respectively. The inhibition types of these three fungicides were found to be non-competitive inhibition with the Ki values of 1.158, 0.638, and 0.145 mM and IC50 values of 0.573, 0.158, 0.010 mM, respectively. The results of in vivo experiments also showed that benomyl, captan and chlorothalonil caused 15.25, 1.96, and 36.70% activity decreases after 24-h treatments compared to that of the control.

Published

2014

43. Purification, crystallization and phase determination of the DR1998 haem b catalase from Deinococcus radiodurans.

Author

Borges PT, Miranda CS, Santos SP, Carita JN, Frazão C, and Romão CV

Subjects

Catalase isolation & purification, Crystallization, Heme isolation & purification, Protein Structure, Tertiary, Catalase chemistry, Deinococcus enzymology, Heme chemistry

Abstract

The protective mechanisms of Deinococcus radiodurans against primary reactive oxygen species involve nonenzymatic scavengers and a powerful enzymatic antioxidant system including catalases, peroxidases and superoxide dismutases that prevents oxidative damage. Catalase is an enzyme that is responsible for the conversion of H2O2 to O2 and H2O, protecting the organism from the oxidative effect of H2O2. This study reports the purification and crystallization of the DR1998 catalase from D. radiodurans. The crystals diffracted to 2.6 Å resolution and belonged to space group C2221, with unit-cell parameters a = 97.33, b = 311.88, c = 145.63 Å, suggesting that they contain four molecules per asymmetric unit. The initial phases were determined by molecular replacement and the obtained solution shows the typical catalase quaternary structure. A preliminary model of the protein structure has been built and refinement is currently in progress.

Published

2014

44. Immunodetection of a brown planthopper (Nilaparvata lugens Stål) salivary catalase-like protein into tissues of rice, Oryza sativa.

Author

Petrova A and Smith CM

Subjects

Animals, Catalase immunology, Gene Expression, Hemiptera pathogenicity, Hydrogen Peroxide metabolism, Oryza enzymology, Oryza parasitology, Pest Control, Plant Diseases, Saliva enzymology, Catalase isolation & purification, Host-Parasite Interactions genetics, Salivary Glands metabolism

Abstract

Saliva plays an important role in host plant-phloem-feeding insect molecular interactions. To better elucidate the role of insect saliva, a series of experiments were conducted to establish if catalase from the salivary glands of the brown planthopper (BPH; Nilaparvata lugens Stål) was secreted into rice host plant tissue during feeding. Catalase is the main enzyme that decomposes hydrogen peroxide (H2O2) at high concentrations. H2O2 is a part of the free radicals system that mediates important physiological roles including signalling and defence. Previous studies have suggested that H2O2 is involved in the rice endogenous response to BPH feeding. If, the BPH secretes catalase into host plant tissue this will counter the effects of H2O2, from detoxification to interfering with plant signalling and defence mechanisms. When BPHs were fed on a hopper-resistant rice variety for 24 h, catalase activity in the salivary glands increased 3.5-fold compared with hoppers fed on a susceptible rice variety. Further supporting evidence of the effects of BPH catalase was demonstrated by immunodetection analyses where results from two independent sources: BPH-infested rice tissue and BPH-probed artificial diets, suggest that the BPH secretes catalase-like protein during feeding. The possible physiological roles of BPH-secreted catalase are discussed., (© 2013 The Royal Entomological Society.)

Published

2014

45. Purification of recombinant catalase-peroxidase HPI from E. coli and its application in enzymatic polymerization reactions.

Author

Di Gennaro P, Bargna A, Bruno F, and Sello G

Subjects

Aniline Compounds metabolism, Catalase genetics, Chromatography, High Pressure Liquid, Escherichia coli Proteins genetics, Phenols metabolism, Polymerization, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Biopolymers metabolism, Catalase isolation & purification, Catalase metabolism, Escherichia coli enzymology, Escherichia coli genetics, Escherichia coli Proteins isolation & purification, Escherichia coli Proteins metabolism

Abstract

In this paper, a recombinant catalase-peroxidase HPI from Escherichia coli was prepared, purified, and used in enzymatic polymerization reactions for the production of several oligomeric products. We tested the enzyme on four different substrates, chosen as representative of phenols and anilines: phenol, 3-methoxyphenol, catechol, and aniline. The polymerization reactions were followed by SEC-HPLC analysis, and except for aniline, all the other substrates were completely converted into one or more polymerization products. Results showed that reactions performed with phenol and 3-methoxyphenol allowed the isolation of some oligomers of different weight: a 27-monomeric unit oligomer and a 23-U oligomer are the heaviest ones. Experiments performed with catechol showed the formation of oligomers of 7 U in the reaction with HPI. HPI polymerization reactions performed with aniline allowed the identification of two different oligomers, one of 4 U and one of 10 U. All the substrates have been also used in reactions catalyzed by HRP in the same reaction conditions. Several products were common to the two enzymes. This work suggests the use of HPI as an alternative enzyme in peroxidatic reactions for the production of different oligomers from phenols and other compounds.

Published

2014

46. Purification and characterization of catalase from marine bacterium Acinetobacter sp. YS0810.

Author

Fu X, Wang W, Hao J, Zhu X, and Sun M

Subjects

Amino Acid Sequence, Catalase chemistry, Catalase genetics, Chromatography, Gel, Hydrogen-Ion Concentration, Substrate Specificity, Acinetobacter enzymology, Aquatic Organisms enzymology, Catalase isolation & purification

Abstract

The catalase from marine bacterium Acinetobacter sp. YS0810 (YS0810CAT) was purified and characterized. Consecutive steps were used to achieve the purified enzyme as follows: ethanol precipitation, DEAE Sepharose ion exchange, Superdex 200 gel filtration, and Resource Q ion exchange. The active enzyme consisted of four identical subunits of 57.256 kDa. It showed a Soret peak at 405 nm, indicating the presence of iron protoporphyrin IX. The catalase was not apparently reduced by sodium dithionite but was inhibited by 3-amino-1,2,4-triazole, hydroxylamine hydrochloride, and sodium azide. Peroxidase-like activity was not found with the substrate o-phenylenediamine. So the catalase was determined to be a monofunctional catalase. N-terminal amino acid of the catalase analysis gave the sequence SQDPKKCPVTHLTTE, which showed high degree of homology with those of known catalases from bacteria. The analysis of amino acid sequence of the purified catalase by matrix-assisted laser desorption ionization time-of-flight mass spectrometry showed that it was a new catalase, in spite of its high homology with those of known catalases from other bacteria. The catalase showed high alkali stability and thermostability.

Published

2014

47. Purification and cloning of nicosulfuron-degrading enzymes from Bacillus subtilis YB1.

Author

Kang ZH, Ren CC, Zhang JL, Dong JG, Li X, and Wei XJ

Subjects

ATP-Binding Cassette Transporters chemistry, ATP-Binding Cassette Transporters genetics, Acetoin Dehydrogenase chemistry, Acetoin Dehydrogenase genetics, Bacillus subtilis enzymology, Bacillus subtilis genetics, Bacterial Proteins chemistry, Bacterial Proteins genetics, Biodegradation, Environmental, Catalase chemistry, Catalase genetics, Chromatography, Ion Exchange, Cloning, Molecular, Environmental Pollutants chemistry, Escherichia coli genetics, Escherichia coli metabolism, Herbicides chemistry, Molecular Weight, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, ATP-Binding Cassette Transporters isolation & purification, Acetoin Dehydrogenase isolation & purification, Bacillus subtilis chemistry, Bacterial Proteins isolation & purification, Catalase isolation & purification, Pyridines chemistry, Sulfonylurea Compounds chemistry

Abstract

The nicosulfuron-degrading enzymes from Bacillus subtilis strain YB1 were purified and their genes were cloned. The proteins of bacterial culture filtrate were precipitated with ammonium sulfate or acetone. The extracellular proteins concentrated by acetone were purified from DEAE-Sepharose Fast Flow chromatography. The four protein peaks eluted from DEAE-column were separated and purified by native PAGE. Three components (P1-1, P3-2, P4-3) had nicosulfuron-degrading activity, and component P4-3 degradated 57.5% of this compound. The molecular weights of the components were 33.5, 54.8 and 37.0 kDa, respectively. The amino acid sequences of nicosulfuron-degrading enzymes from B. subtilis YB1 were determined by MALDI-TOF-MS, indicating these enzymes as manganese ABC transporter, vegetative catalase 1 and acetoin dehydrogenase E1, respectively. Using PCR amplification, genes 918, 1428, 1026 bp in size were detected for the enzymes studied.

Published

2014

48. Purification, crystallization and preliminary crystallographic analysis of KatB, a manganese catalase from Anabaena PCC 7120.

Author

Bihani SC, Chakravarty D, and Ballal A

Subjects

Crystallization, Crystallography, X-Ray, Electrophoresis, Polyacrylamide Gel, Anabaena enzymology, Bacterial Proteins chemistry, Bacterial Proteins isolation & purification, Catalase chemistry, Catalase isolation & purification

Abstract

Catalases are enzymes that play an important role in the detoxification of hydrogen peroxide (H2O2) in aerobic organisms. Among catalases, haem-containing catalases are ubiquitously distributed and their enzymatic mechanism is very well understood. On the other hand, manganese catalases that contain a bimanganese core in the active site have been less well characterized and their mode of action is not fully understood. The genome of Anabaena PCC 7120 does not show the presence of a haem catalase-like gene; instead, two ORFs encoding manganese catalases (Mn-catalases) are present. Here, the crystallization and preliminary X-ray crystallographic analysis of KatB, one of the two Mn-catalases from Anabaena, are reported. KatB was crystallized using the hanging-drop vapour-diffusion method with PEG 400 as a precipitant and calcium acetate as an additive. Diffraction data were collected in-house on an Agilent SuperNova system using a microfocus sealed-tube X-ray source. The crystal diffracted to 2.2 Å resolution at 100 K. The tetragonal crystal belonged to space group P4(1)2(1)2 (or enantiomer), with unit-cell parameters a = b = 101.87, c = 138.86 Å. Preliminary X-ray diffraction analysis using the Matthews coefficient and self-rotation function suggests the presence of a trimer in the asymmetric unit.

Published

2013

49. Three-phase partitioning as a rapid and easy method for the purification and recovery of catalase from sweet potato tubers (Solanum tuberosum).

Author

Duman YA and Kaya E

Subjects

Catalase analysis, Enzyme Activation, Enzyme Stability, Molecular Weight, Catalase chemistry, Catalase isolation & purification, Liquid-Liquid Extraction methods, Plant Tubers enzymology, Solanum tuberosum enzymology

Abstract

Three-phase partitioning (TPP) was used to purify and recover catalase from potato crude extract. The method consists of ammonium sulfate saturation, t-butanol addition, and adjustment of pH, respectively. The best catalase recovery (262 %) and 14.1-fold purification were seen in the interfacial phase in the presence of 40 % (w/v) ammonium sulfate saturation with 1.0:1.0 crude extract/t-butanol ratio (v/v) at pH 7 in a single step. The sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) analysis of the enzyme showed comparatively purification and protein molecular weight was nearly found to be 56 kDa. This study shows that TPP is a simple, economical, and quick method for the recovering of catalase and can be used for the purification process.

Published

2013

50. Catalase and superoxide dismutase activities and the total protein content of protocorm-like bodies of Dendrobium sonia-28 subjected to vitrification.

Author

Poobathy R, Sinniah UR, Xavier R, and Subramaniam S

Subjects

Catalase isolation & purification, Enzyme Activation, Plant Proteins isolation & purification, Superoxide Dismutase isolation & purification, Vitrification, Catalase chemistry, Dendrobium chemistry, Dendrobium embryology, Plant Proteins chemistry, Seeds chemistry, Superoxide Dismutase chemistry

Abstract

Dendrobium sonia-28 is an important ornamental orchid in the Malaysian flower industry. However, the genus faces both low germination rates and the risk of producing heterozygous progenies. Cryopreservation is currently the favoured long-term storage method for orchids with propagation problems. Vitrification, a frequently used cryopreservation technique, involves the application of pretreatments and cryoprotectants to protect and recover explants during and after storage in liquid nitrogen. However, cryopreservation may cause osmotic injuries and toxicity to cryopreserved explants from the use of highly concentrated additives, and cellular injuries from thawing, devitrification and ice formation. Reactive oxygen species (ROS), occurring during dehydration and cryopreservation, may also cause membrane damage. Plants possess efficient antioxidant systems such as the superoxide dismutase (SOD) and catalase (CAT) enzymes to scavenge ROS during low temperature stress. In this study, protocorm-like bodies (PLBs) of Dendrobium sonia-28 were assayed for the total protein content, and both SOD and CAT activities, at each stage of a vitrification exercise to observe for deleterious stages in the protocol. The results indicated that cryopreserved PLBs of Dendrobium sonia-28 underwent excessive post-thawing oxidative stress due to decreased levels of the CAT enzyme at the post-thawing recovery stage, which contributed to the poor survival rates of the cryopreserved PLBs.

Published

2013