Your search keyword '"Hopper D"' showing total 19 results

1. Lupanine hydroxylase, a quinocytochrome c from an alkaloid-degrading Pseudomonas sp.

Author

Hopper DJ, Rogozinski J, and Toczko M

Subjects

Chromatography, Gel, Coenzymes metabolism, Electrophoresis, Polyacrylamide Gel, Hydroxylation, Isoelectric Focusing, Kinetics, Mixed Function Oxygenases metabolism, PQQ Cofactor, Pseudomonas growth & development, Quinolones metabolism, Spectrum Analysis, Substrate Specificity, Mixed Function Oxygenases isolation & purification, Oxidoreductases Acting on CH-NH Group Donors, Pseudomonas enzymology

Abstract

Lupanine 17-hydroxylase, the first enzyme in the pathway for bacterial degradation of the alkaloid, lupanine, was purified from a Pseudomonas sp. The enzyme acts by initial dehydrogenation of the substrate, and cytochrome c was used as electron acceptor in assays. It had an Mr of 66,000 by ultracentrifuge studies and 74,000 by gel filtration. The visible absorption spectrum was that of a cytochrome c, and a stoicheiometry of one haem group per molecule of enzyme was calculated. SDS/PAGE gave a single band of Mr 72,000 containing the haem group. The enzyme also contained pyrroloquinoline quinone (PQQ), which could be removed by isoelectric focusing. The apoenzyme was reconstituted to full activity with addition of PQQ, and a stoicheiometry of one molecule of PQQ per molecule of enzyme was calculated. Steady-state kinetics gave values of 3.6 microM for the Km for lupanine, 21.3 microM for the Km for cytochrome c and 217 s-1 for the Kcat.

Published

1991

2. p-cresol methylhydroxylase from a denitrifying bacterium involved in anaerobic degradation of p-cresol.

Author

Hopper DJ, Bossert ID, and Rhodes-Roberts ME

Subjects

Anaerobiosis, Cytochromes metabolism, Flavoproteins metabolism, Kinetics, Mixed Function Oxygenases isolation & purification, Oxidation-Reduction, Spectrophotometry, Ultraviolet, Alcaligenes enzymology, Cresols metabolism, Mixed Function Oxygenases metabolism

Abstract

A bacterium, strain PC-07, previously isolated as part of a coculture capable of growing on p-cresol under anaerobic conditions with nitrate as the acceptor was identified as an Achromobacter sp. The first enzyme of the pathway, p-cresol methylhydroxylase, which converts its substrate into p-hydroxybenzyl alcohol, was purified. The enzyme had an Mr of 130,000 and the spectrum of a flavocytochrome. It was composed of flavoprotein subunits of Mr 54,000 and cytochrome subunits of Mr 12,500. The midpoint redox potential of the cytochrome was 232 mV. The Km and kcat for p-cresol were 21 microM and 112 s-1 respectively, and the Km for phenazine methosulfate, the artificial acceptor used in the assays, was determined to be 1.7 mM. These properties place the enzyme in the same class as the p-cresol methylhydroxylases from aerobically isolated Pseudomonas spp.

Published

1991

3. Stereochemical aspects of the oxidation of 4-ethylphenol by the bacterial enzyme 4-ethylphenol methylenehydroxylase.

Author

Reeve CD, Carver MA, and Hopper DJ

Subjects

Alcohol Oxidoreductases metabolism, Bacterial Proteins metabolism, Oxidation-Reduction, Phenylethyl Alcohol analogs & derivatives, Phenylethyl Alcohol metabolism, Pseudomonas enzymology, Stereoisomerism, Mixed Function Oxygenases metabolism, Phenols metabolism

Abstract

The O2-independent hydroxylase 4-ethylphenol methylenehydroxylase (4EPMH) from Pseudomonas putida JD1 catalysed the complete conversion of 4-ethylphenol into 1-(4-hydroxyphenyl)ethanol together with a small amount of 4-hydroxyacetophenone, but with no formation of the side product 4-vinylphenol reported to be formed when the similar enzyme p-cresol methylhydroxylase (PCMH) catalyses this reaction. The enantiomer of 1-(4-hydroxyphenyl)ethanol produced by 4EPMH was R(+) when horse heart cytochrome c or azurin was used as electron acceptor for the enzyme. PCMHs from various bacterial strains produced the S(-)-alcohol. Both enantiomers of 1-(4-hydroxyphenyl)ethanol were substrates for conversion into 4-hydroxyacetophenone by 4EPMH, but the S(-)-isomer was preferred. The Km and kcat. were 1.2 mM and 41 s-1 respectively for the S(-)-alcohol and 4.7 mM and 22 s-1 for the R(+)-alcohol. In addition to the 1-(4-hydroxyphenyl)ethanol dehydrogenase activity of 4-EPMH, NAD(+)-linked dehydrogenase activity for both enantiomers of the alcohol was found in extracts of Ps. putida JD1.

Published

1990

4. Formation and properties of flavoprotein-cytochrome hybrids by recombination of subunits from different species.

Author

Koerber SC, Hopper DJ, McIntire WS, and Singer TP

Subjects

Cytochromes isolation & purification, Isoenzymes isolation & purification, Kinetics, Mixed Function Oxygenases isolation & purification, Protein Multimerization, Species Specificity, Cytochromes metabolism, Flavoproteins metabolism, Isoenzymes metabolism, Mixed Function Oxygenases metabolism, Pseudomonas enzymology

Abstract

p-Cresol methylhydroxylases from four different pseudomonads differ in their isoelectric points and, to a lesser extent, in Mr values and substrate specificity. The enzymes from three species were isolated in homogeneous form, then resolved into their flavoprotein and cytochrome subunits, and the subunits were recombined to yield the nine possible hybrids (i.e. three intraspecies and six interspecies). The resulting flavocytochromes showed extensive similarities in steady-state kinetic parameters and in the dissociation constants of their subunits. Evidence is also presented that a fourth type of p-cresol methylhydroxylase, from Pseudomonas putida (N.C.I.B. 9869, form 'B'), the subunits of which cannot be isolated by the isoelectric focusing technique used to separate the subunits of the other flavocytochromes, nevertheless dissociates slowly at high dilution. The dissociation is reflected by a decline of catalytic activity with time. This process for the 'B' enzyme is prevented by the presence of substrate or an excess of a cytochrome subunit isolated from another enzyme species. Incubation of the dissociated subunits with p-cresol brings about extensive, albeit incomplete, re-association and regeneration of activity.

Published

1985

5. P-cresol and 3,5-xylenol methylhydroxylases in Pseudomonas putida N.C.I.B. 9896.

Author

Keat MJ and Hopper DJ

Subjects

Cresols, Electrophoresis, Polyacrylamide Gel, Flavins analysis, Kinetics, Mixed Function Oxygenases isolation & purification, Oxidation-Reduction, Substrate Specificity, Xylenes, Mixed Function Oxygenases metabolism, Pseudomonas enzymology

Abstract

Pseudomonas putida N.C.I.B. 9869, when grown on 3,5-xylenol, hydroxylates the methyl groups on 3,5-xylenol and on p-cresol by two different enzymes. 3,5-Xylenol methylhydroxylase, studied only in relatively crude extracts, requires NADH, is not active with p-cresol and is inhibited by cyanide, but not by CO. The p-cresol methylhydroxylase requires an electron acceptor and will act under anaerobic conditions. It was purified and is a flavocytochrome c of mol.wt. approx. 114,000 consisting of two subunits of equal size. The enzyme catalyses the hydroxylation of p-cresol (Km 16 micron) and the further oxidation of product, p-hydroxybenzyl alcohol (Km 27 micron) to p-hydroxybenzaldehyde. A different p-cresol methylhydroxylase of the flavocytochrome c type is induced by growth on p-cresol. It too was purified and has mol.wt. approx. 100,000, and again consisted of two equal-size subunits. The Km for p=cresol 3.6 micron and for p=hydroxybenzyl alcohol, 15 micron.

Published

1978

6. Periplasmic location of p-cresol methylhydroxylase in Pseudomonas putida.

Author

Hopper DJ, Jones MR, and Causer MJ

Subjects

Azurin analysis, Cell Membrane enzymology, Cell Wall enzymology, Cytoplasm enzymology, Edetic Acid pharmacology, Muramidase pharmacology, Pseudomonas drug effects, Spheroplasts enzymology, Mixed Function Oxygenases analysis, Pseudomonas enzymology, Subcellular Fractions enzymology

Abstract

The cellular location of the flavocytochrome c, p-cresol methylhydroxylase was investigated in two strains of Pseudomonas putida. In both cases the enzymes were shown to be located in the periplasmic fraction by their release during treatment of the bacteria with EDTA and lysozyme in a solution containing a high concentration of sucrose. For strain NCIB 9869 the finding is in accord with the suggestion that the physiological acceptor for the enzyme is azurin as this too was shown to be located mostly in the periplasm.

Published

1985

7. 8 alpha-(O-Tyrosyl)flavin adenine dinucleotide, the prosthetic group of bacterial p-cresol methylhydroxylase.

Author

McIntire W, Edmondson DE, Hopper DJ, and Singer TP

Subjects

Cresols analysis, Flavin-Adenine Dinucleotide analysis, Flavin-Adenine Dinucleotide chemical synthesis, Magnetic Resonance Spectroscopy, Peptide Fragments analysis, Spectrometry, Fluorescence, Spectrophotometry, Flavin-Adenine Dinucleotide analogs & derivatives, Mixed Function Oxygenases analysis, Pseudomonas enzymology

Abstract

8 alpha-(O-Tyrosyl)riboflavin has been synthesized by condensation of the copper complex of L-tyrosine with 8 alpha-bromotetraacetylriboflavin. The structure of this synthetic product was proven by absorption and 1H NMR spectroscopy and by chemical degradation, which yielded 1 mol of tyrosine per mol of flavin. The synthetic compound comigrated wtih the (aminoacyl)riboflavin isolated from the p-cresol methylhydroxylase of Pseudomonas putida, and both showed identical absorption and fluorescence spectral properties. 8 alpha-(O-Tyrosyl)riboflavin as well as the flavin-containing decapeptide from p-cresol methylhydroxylase undergoes reductive cleavage to form riboflavin and FAD, respectively, on anaerobic treatment with dithionite. In contrast, the native enzyme, on reduction with dithionite, yields a reduced flavin via a red (anionic) flavosemiquinone intermediate, which remains covalently bound to the protein even under denaturing conditions. 8 alpha-(O-Tyrosyl)riboflavin bound to apoflavodoxin is also not cleaved on reduction with dithionite, but, instead, a blue (neutral) semiquinone of tyrosylriboflavin is generated, which is resistant to further reduction with dithionite. Three p-cresol methylhydroxylases, isolated from different strains of Pseudomonas putida, differing in molecular weight and Km values for substrates, contain the same peptide at the flavin site. These data provide definitive proof for the existence of 8 alpha-(O-tyrosyl)riboflavin in nature.

Published

1981

8. Preliminary X-ray study of p-cresol methylhydroxylase (flavocytochrome c) from Pseudomonas putida N.C.I.B. 9869.

Author

Shamala N, Lim LW, Mathews FS, McIntire W, Singer TP, and Hopper DJ

Subjects

X-Ray Diffraction, Mixed Function Oxygenases, Pseudomonas enzymology

Abstract

Single crystals of p-cresol methylhydroxylase, a flavocytochrome c from Pseudomonas putida, have been prepared. The crystals are orthorhombic, space group P212121 with unit cell parameters; a = 140.3 A, b = 130.6 A and c = 74.1 A. They contain a single non-symmetric dimer per asymmetric unit and diffract to at least 2.5 A resolution.

Published

1985

9. Incorporation of [18O]water in the formation of p-hydroxybenzyl alcohol by the p-cresol methylhydroxylase from Pseudomonas putida.

Author

Hopper DJ

Subjects

Chemical Phenomena, Chemistry, Cresols, Benzyl Alcohols metabolism, Benzyl Compounds metabolism, Mixed Function Oxygenases metabolism, Pseudomonas enzymology, Water metabolism

Abstract

In the hydroxylation of the methyl group of p-cresol by an enzyme from Pseudomonas putida the oxygen atom is derived from water. Although a second reaction by the same enzyme converts the product, p-hydroxybenzyl alcohol, into the aldehyde, the alcohol is an enzyme-free intermediate.

Published

1978

10. 8 alpha-O-Tyrosyl-FAD: a new form of covalently bound flavin from p-cresol methylhydroxylase.

Author

McIntire W, Edmondson DE, Singer TP, and Hopper DJ

Subjects

Amino Acids analysis, Cresols isolation & purification, Cresols metabolism, Dansyl Compounds, Flavin-Adenine Dinucleotide analysis, Spectrometry, Fluorescence, Spectrophotometry, Flavin-Adenine Dinucleotide analogs & derivatives, Mixed Function Oxygenases isolation & purification, Mixed Function Oxygenases metabolism, Pseudomonas enzymology

Published

1980

11. Regulation of enzymes of the 3,5-xylenol-degradative pathway in Pseudomonas putida: evidence for a plasmid.

Author

Hopper DJ and Kemp PD

Subjects

Alcohol Oxidoreductases metabolism, Aldehyde Oxidoreductases metabolism, Cresols metabolism, Hydroxybenzoates metabolism, Mixed Function Oxygenases biosynthesis, Pseudomonas genetics, Mixed Function Oxygenases metabolism, Plasmids, Pseudomonas enzymology, Xylenes metabolism

Abstract

Constitutive synthesis of enzymes responsible for methyl group oxidation in 3,5-xylenol degradation and an associated p-cresol methylhydroxylase in Pseudomonas putida NCIB 9869 was shown by their retention at high specific activities in cells transferred from 3,5-xylenol medium to glutamate medium. The specific activities of other enzymes of the 3,5-xylenol pathway declined upon removal of aromatic substrate, consistent with their inducible control. Specific activities of the methyl-oxidizing enzymes showed an eventual decline concomitant with a decrease in the fraction of bacteria capable of growth with 3,5-xylenol; a simultaneous loss of the ability to grow with m-hydroxybenzoate was also observed. The property of 3,5-xylenol utilization could be transferred to another strain of P. putida. It is proposed that enzymes of the 3,5-xylenol pathway and those for conversion of p-cresol to p-hydroxybenzoate are plasmid encoded, that the early methyl-oxidizing enzymes are expressed constitutively, and that the later enzymes are inducible.

Published

1980

12. The hydroxylation of P-cresol and its conversion to P-hydroxybenzaldehyde in Pseudomonas putida.

Author

Hopper DJ

Subjects

Anaerobiosis, Kinetics, Mixed Function Oxygenases isolation & purification, Cresols metabolism, Mixed Function Oxygenases metabolism, Pseudomonas metabolism

Published

1976

13. p-Cresol methylhydroxylase. Assay and general properties.

Author

McIntire W, Hopper DJ, and Singer TP

Subjects

Benzyl Alcohols metabolism, Cresols metabolism, Cytochrome c Group metabolism, Hydrogen-Ion Concentration, Kinetics, Methylphenazonium Methosulfate metabolism, Osmolar Concentration, Pseudomonas enzymology, Spectrophotometry, Substrate Specificity, Mixed Function Oxygenases metabolism

Abstract

p-Cresol methylhydroxylase from Pseudomonas putida, an anaerobic dehydrogenase that catalyses the oxidation of p-cresol to p-hydroxybenzyl alcohol and then to p-hydroxybenzaldehyde, is an enzyme of great interest in several respects. One of these is the fact that its flavoprotein and cytochrome c subunits may be reversibly dissociated with ease, with full regeneration of the activity and its native properties on recombining the components. Bisubstrate kinetic analysis of the unresolved enzyme gives parallel-line kinetics in double-reciprocal plots, whereas the reaction of the separated flavoprotein subunit with substrates is described by converging lines. The mechanistic implications of these behaviours are discussed. Reductive titration with dithionite results in the uptake of 3 electrons by the enzyme, with the intermediate formation of the anionic flavin radical [McIntire, Edmondson, Hopper & Singer (1981) Biochemistry 20, 3068-3075]. Reductive titration with substrates resulted initially only in reduction of the cytochrome subunit, followed by formation of the anionic radical and finally the fully reduced enzyme. These observations suggest rapid intermolecular electron transfer between p-cresol methylhydroxylase molecules. This paper also examines the effect of pH and ionic strength on the activity and specificity of the enzyme with respect to substrates and natural, as well as artificial, electron acceptors. The absorption coefficients of the enzyme and of its subunits in various oxidation states are also presented.

Published

1985

14. Redox potential of the cytochrome c in the flavocytochrome p-cresol methylhydroxylase.

Author

Hopper DJ

Subjects

Kinetics, Macromolecular Substances, Oxidation-Reduction, Species Specificity, Cytochrome c Group metabolism, Mixed Function Oxygenases metabolism, Pseudomonas enzymology

Abstract

The redox potential of the cytochrome c in 5 flavocytochrome c proteins, all p-cresol methylhydroxylases purified from species of Pseudomonas, was measured. All gave similar values ranging from 226-250 mV. Two of the enzymes, from Pseudomonas putida NC1B 9866 and NC1B 9869, were resolved into their flavoprotein and cytochrome subunits and the redox potentials of the isolated cytochrome c subunits measured. The values for these were 60-70 mV below those for the whole enzymes but, in both cases, reconstitution of active enzyme by addition of the flavoprotein subunit restored the original potential.

Published

1983

15. Stereochemistry of 1-(4'-hydroxyphenyl)ethanol produced by hydroxylation of 4-ethylphenol by p-cresol methylhydroxylase.

Author

McIntire W, Hopper DJ, Craig JC, Everhart ET, Webster RV, Causer MJ, and Singer TP

Subjects

Hydroxylation, Molecular Conformation, Phenylethyl Alcohol metabolism, Pseudomonas metabolism, Stereoisomerism, Ethanol analogs & derivatives, Mixed Function Oxygenases metabolism, Phenols metabolism, Phenylethyl Alcohol analogs & derivatives

Abstract

Enzymic hydroxylation of 4-ethylphenol by (a) Pseudomonas putida and (b) highly purified p-cresol methylhydroxylase gave optically active 1-(4'-hydroxyphenyl)-ethanol. The products were transformed into the phenolic methyl ethers and shown to contain 69.5% and 65.6%, respectively, of the (S)-(-)-isomer. The stereochemistry of the reaction is discussed in terms of three distinct steps occurring at the active site of the enzyme.

Published

1984

16. Steady-state and stopped-flow kinetic measurements of the primary deuterium isotope effect in the reaction catalyzed by p-cresol methylhydroxylase.

Author

McIntire WS, Hopper DJ, and Singer TP

Subjects

Binding Sites, Deuterium pharmacology, Flavoproteins metabolism, Mathematics, Mixed Function Oxygenases pharmacology, Phenols metabolism, Protein Conformation, Pseudomonas enzymology, Spectrometry, Fluorescence methods, Deuterium pharmacokinetics, Mixed Function Oxygenases pharmacokinetics

Abstract

Steady-state kinetic studies for the reaction of the flavocytochrome p-cresol methylhydroxylase with the reducing substrates (S) p-cresol, 4-ethylphenol, and their corresponding alpha-deuteriated analogues are presented. The results from these experiments and those from studies involving various reoxidizing substrates support the proposed apparent ping-pong mechanism. With phenazine methosulfate (PMS) as the reoxidant for studies at pH 7.6 and 6 or 25 degrees C, the isotope effects on kcat are lower than the intrinsic isotope effect. The values for D(kcat/KS) are equal to the intrinsic effect for p-cresol at 25 degrees C and for 4-ethylphenol at both 6 and 25 degrees C. However, the value for this steady-state parameter at 6 degrees C for p-cresol is lower than the intrinsic effect. The values for D(kcat/KPMS) are nearly equal to 1.0 under all conditions. In contrast, the steady-state kinetic analysis for the isolated flavoprotein subunit of p-cresol methylhydroxylase involving p-cresol and PMS as substrates indicates that a random-binding mechanism is operating. Additionally, several of the steady-state parameters yield values for the apparent intrinsic isotope effect for the flavoprotein. The results of stopped-flow kinetic studies are also reported. At pH 7.6 the intrinsic isotope effect (Dk2) for the reduction of the enzyme by 4-ethylphenol is 4.8-5.0 at 25 degrees C and 4.0 at 6 degrees C. This technique yields a value for Dk2 of 7.05 at 6 degrees C and pH 7.6 for p-cresol.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1987

17. The purification and properties of 4-hydroxyisophthalate hydroxylase from Pseudomonas putida NCIB 9866.

Author

Elmorsi EA and Hopper DJ

Subjects

4-Hydroxybenzoate-3-Monooxygenase metabolism, Apoenzymes, Catechin metabolism, Flavin-Adenine Dinucleotide analysis, Hydrogen-Ion Concentration, Mixed Function Oxygenases antagonists & inhibitors, Mixed Function Oxygenases metabolism, Molecular Weight, NAD pharmacology, NADP pharmacology, Phthalic Acids metabolism, Structure-Activity Relationship, Sulfhydryl Reagents pharmacology, Mixed Function Oxygenases isolation & purification, Pseudomonas enzymology

Published

1977

18. The purification and properties of p-cresol-(acceptor) oxidoreductase (hydroxylating), a flavocytochrome from Pseudomonas putida.

Author

Hopper DJ and Taylor DG

Subjects

Cresols, Cytochromes, Flavins analysis, Heme analysis, Kinetics, Molecular Weight, Proteins analysis, Spectrum Analysis, Mixed Function Oxygenases isolation & purification, Pseudomonas enzymology

Abstract

The enzyme that catalyses the hydroxylation of the methyl group of p-cresol was purified from Pseudomonas putida. It has mol.wt. 115000 and appears to contain two subunits of equal molecular weight. One subunit is a c-type cytochrome and the other is a flavoprotein. Reduction of the cytochrome occurred on addition of substrate. The same enzyme catalyses both p-cresol hydroxylation and the further oxidation of the product, 4-hydroxybenzyl alcohol. The stoicheiometry of acceptor reduced per molecule of substrate oxidized is that for two dehydrogenation reactions. The Km for p-cresol is 7.3 x 10(-6) M and that for 4-hydroxybenzyl alcohol is 47.6 x 10(-6) M. The enzyme, which is assayed with phenazine methosulphate as electron acceptor, was stimulated by particulate material, which probably contains the acceptor in vivo.

Published

1977

19. Properties of 5-hydroxyisophthalate 4-hydroxylase from a coryneform bacteria.

Author

Elmorsi EA and Hopper DJ

Subjects

Flavin-Adenine Dinucleotide metabolism, Flavoproteins metabolism, NADP metabolism, Phthalic Acids, Actinomycetales enzymology, Mixed Function Oxygenases metabolism

Published

1978