Your search keyword '"Urate Oxidase metabolism"' showing total 7 results

1. Modified colorimetric assay for uricase activity and a screen for mutant Bacillus subtilis uricase genes following StEP mutagenesis.

Author

Huang SH and Wu TK

Subjects

Amino Acid Sequence, Bacillus subtilis enzymology, Base Sequence, DNA Primers, Molecular Sequence Data, Mutagenesis, Sequence Homology, Amino Acid, Urate Oxidase chemistry, Bacillus subtilis genetics, Colorimetry methods, Urate Oxidase genetics, Urate Oxidase metabolism

Abstract

This study describes a modified colorimetric assay for uricase activity in flexible 96-well microtiter plates using the uricase/uric acid/horseradish peroxidase/4-aminoantipyrine/3,5-dichloro-2-hydroxybenzene sulfonate colorimetric reaction. The utility of this assay was demonstrated in a screen for mutant uricase enzymes derived from the uricase gene of the thermophilic bacterium Bacillus subtilis by a modified staggered extension process (StEP) mutagenesis. An Escherichia coli library of StEP-derived uricase mutant clones was screened yielding two identical active mutant uricase genes. Two motifs conserved in eukaryotic and prokaryotic uricases are highly conserved in the mutant uricase. The mutant uricase protein was found to exhibit high uricase activity (13.1 U.mg(-1)). Finally, the modified colorimetric method is much more efficient than the conventional ones and greatly reduces assay time from 4 days to less than 20 h.

Published

2004

2. Urate oxidase is imported into peroxisomes recognizing the C-terminal SKL motif of proteins.

Author

Miura S, Oda T, Funai T, Ito M, Okada Y, and Ichiyama A

Subjects

Amino Acid Sequence, Animals, Base Sequence, Biological Transport, Humans, Molecular Sequence Data, Mutation, Oligodeoxyribonucleotides, Rats, Temperature, Time Factors, Urate Oxidase biosynthesis, Urate Oxidase genetics, Liver metabolism, Microbodies metabolism, Oligopeptides metabolism, Urate Oxidase metabolism

Abstract

Rat liver urate oxidase synthesized from cDNA through coupled transcription and translation was incubated at 26 degrees C for 60 min with purified peroxisomes from rat liver. Urate oxidase was efficiently imported into the peroxisomes, as determined by resistance to externally added proteinase K. The amount of imported urate oxidase increased with time and the import was temperature dependent. A synthetic peptide composed of the C-terminal 10 amino acid residues of acyl-CoA oxidase (the C-terminal tripeptide is Ser-Lys-Leu) inhibited the import of urate oxidase, whereas other peptides, in which the C-terminal Ser-Lys-Leu (SKL) sequence was deleted or mutated, were not effective. Two mutant urate oxidase proteins in which the C-terminal Ser-Arg-Leu (SRL) sequence was deleted or mutated to Ser-Glu-Leu (SEL) were not imported into peroxisomes. With substitution of a lysine residue for arginine in the SRL tripeptide at the C-terminus the import activity was retained. These results show that urate oxidase is important into peroxisomes via a common pathway with acyl-CoA oxidase, and that the C-terminal SRL sequence functions as a peroxisomal-targeting signal.

Published

1994

3. Permeability properties of peroxisomes in digitonin-permeabilized rat hepatocytes. Evidence for free permeability towards a variety of substrates.

Author

Verleur N and Wanders RJ

Subjects

Alcohol Oxidoreductases metabolism, Animals, Cell Membrane Permeability drug effects, D-Amino-Acid Oxidase metabolism, Glutathione metabolism, Liver cytology, Liver drug effects, Liver enzymology, Male, Microbodies drug effects, Microbodies enzymology, Oxidation-Reduction, Rats, Rats, Wistar, Urate Oxidase metabolism, Digitonin pharmacology, Liver metabolism, Microbodies metabolism

Abstract

In order to investigate the permeability properties of rat-liver peroxisomes in situ, we selectively permeabilized hepatocytes with digitonin in a medium mimicking the cytosol. This system permitted us to study the latency of peroxisomal oxidases by means of measurement of their activities in permeabilized compared to disrupted hepatocytes. The activity of peroxisomal oxidases was studied using three different methods: (1) measurement of the oxidase-mediated production of H2O2 in a system containing homovanillic acid, horseradish peroxidase and azide; (2) measurement of the rate of substrate utilization or product formation; (3) measurement of the production of H2O2 via the peroxidative action of catalase in the presence of an excess of methanol. The results obtained depended on which system was used to measure the activity of the different oxidases. Our observations lead us to conclude that method 1 cannot be used for latency studies, whereas methods 2 and 3 are suitable under defined circumstances. Based on the results of methods 2 and 3, we conclude that urate oxidase, L-alpha-hydroxyacid oxidase A and D-amino acid oxidase show no structure-linked latency in digitonin-permeabilized hepatocytes, suggesting that the substrates for these enzymes permeate freely through the peroxisomal membrane.

Published

1993

4. Mitochondria and peroxisomes from the cellular slime mould Dictyostelium discoideum. Isolation techniques and urate oxidase association with peroxisomes.

Author

Parish RW

Subjects

2,6-Dichloroindophenol, Acetylglucosaminidase metabolism, Acid Phosphatase metabolism, Adenylate Kinase metabolism, Alkaline Phosphatase metabolism, Catalase metabolism, Cell Fractionation, Centrifugation, Citrate (si)-Synthase metabolism, Hydrogen-Ion Concentration, Malate Dehydrogenase metabolism, Oxidoreductases metabolism, Polyethylene Glycols, Dictyostelium enzymology, Microbodies enzymology, Mitochondria enzymology, Myxomycetes enzymology, Organoids enzymology, Urate Oxidase metabolism

Abstract

The isolation of cell organelles from Dictyostelium discoideum was attempted using a variety of techniques. Cell homogenization (e.g. Potter-Elvehjem, glass beads) gave poor yields of organelles which were, in addition, exceptionally fragile and unstable in density gradients. An isolation method was developed using Triton X-100 in buffered sorbitol/Ficoll solutions at concentrations optimal for plasma membrane rupture. Immediately following cell lysis the solutions were diluted to sub-optimal Triton X-100 concentrations. Sedimentabilities of malate dehydrogenase, citrate synthetase, urate oxidase and catalase of around 55%, 40%, 35% and 55% respectively could be demonstrated using this method. The organelles were more resistant to breakage during resuspension following differential centrifugation and remained largely intact during density gradient centrifugation. The distribution of adenylate kinase activity in gradients showed that at least half the mitochondria retained an intact outer membrane. The mitochondria and peroxisomes could not be clearly separated using conventional sucrose-Ficoll density gradients. Separation was achieved by incubating the cell homogenate with succinate and a tetrazolium dye (2-p-iodophenyl-3-p-nitrophenyl-5-phenyl monotetrazolium chloride). Succinate dehydrogenase activity of mitochondria reduced the tetrazolium dye and the product (formazan) was deposited on the mitochondrial membranes ("heavy-labelling"). The mitochondria then sedimented to denser regions of the gradient while catalase distribution remained unchanged. The treatment left both organelles intact. The mitochondria (1.21 g/ml) were slightly denser than the peroxisomes (1.19 g/ml). The peroxisomes contained catalase and urate oxidase; no other hydrogen-peroxide-producing oxidases were detected. The slime mould urate oxidase resembled the mammalian enzyme. It had an apparent Km value of 12.5 muM, an optimum of activity at pH 8.5 in borate buffer and was competitively inhibited by trichloropurine.

Published

1975

5. Kinetic studies dealing with an immobilized bienzyme system.

Author

Hervagault JF, Joly G, and Thomas D

Subjects

Binding, Competitive, Diffusion, Kinetics, Permeability, Protein Binding, Serum Albumin, Urate Oxidase antagonists & inhibitors, Xanthines pharmacology, Membranes, Artificial, Urate Oxidase metabolism, Xanthine Oxidase metabolism

Abstract

The binding of enzymes into artificial membranes makes possible a study of the interaction between membrane structure and enzyme kinetics within a simple context. Artificial protein membranes bearing a bienzyme system (xanthine oxidase, uricase) are produced by using a co-crosslinking method. The inhibition of uricase was shown to be dependent not only on the concentration of inhibitor in the bulk solution, but also on the kinetic properties of the membrane-bound enzymes. In the presence of xanthine oxidase inside the structure the uricase inhibition by xanthine is less important than in solution. Under defined conditions the activity was found to be higher in the presence of inhibitor than in its absence. Due to diffusion limitations this specific bienzyme system is more efficient when immobilized inside a membrane than when in solution.

Published

1975

6. Urate oxidase and its association with peroxisomes in Acanthamoeba sp.

Author

Müller M and Moller KM

Subjects

Amoeba cytology, Catalase, Centrifugation, Density Gradient, Cyanides pharmacology, Depression, Chemical, Electron Transport, Hydrogen Peroxide metabolism, Hydrogen-Ion Concentration, Purines pharmacology, Urate Oxidase antagonists & inhibitors, Amoeba enzymology, Microsomes, Urate Oxidase metabolism

Published

1969

7. Urate oxidase in primate phylogenesis.

Author

Christen P, Peacock WC, Christen AE, and Wacker WE

Subjects

Animals, Biological Evolution, Creatinine urine, Drug Stability, Fasting, Haplorhini, Humans, Primates, Purines metabolism, Species Specificity, Uric Acid blood, Uric Acid urine, Liver enzymology, Urate Oxidase metabolism, Uric Acid metabolism

Published

1970