Your search keyword '"Hopper, David J."' showing total 8 results

1. Genome Sequence Analysis of Two Pseudomonas putida Strains to Identify a 17-Hydroxylase Putatively Involved in Sparteine Degradation.

Author

Detheridge AP, Griffith GW, and Hopper DJ

Subjects

Alkaloids genetics, Oxidoreductases Acting on CH-NH Group Donors genetics, Sequence Analysis methods, Sparteine analogs & derivatives, Whole Genome Sequencing methods, Bacterial Proteins genetics, Genome, Bacterial genetics, Pseudomonas putida genetics, Sparteine genetics, Steroid 17-alpha-Hydroxylase genetics

Abstract

Two strains of Pseudomonas putida, Psp-LUP and Psp-SPAR, capable of growth on the quinolizidine alkaloids, lupanine and sparteine respectively, were studied here. We report the isolation of Psp-SPAR and the complete genome sequencing of both bacteria. Both were confirmed to belong to P. putida, Psp-LUP close to the type isolate of the species (NBRC14164 T ) and Psp-SPAR close to strains KT2440 and F1. Psp-SPAR did not grow on lupanine but did contain a gene encoding a putative quinolizidine-17-hydroxylase peptide which exhibited high similarity (76%identity) to the lupanine-17-hydroxylase characterised from Psp-LUP.

Published

2018

2. The 1.1 Å resolution structure of a periplasmic phosphate-binding protein from Stenotrophomonas maltophilia: a crystallization contaminant identified by molecular replacement using the entire Protein Data Bank.

Author

Keegan R, Waterman DG, Hopper DJ, Coates L, Taylor G, Guo J, Coker AR, Erskine PT, Wood SP, and Cooper JB

Subjects

Amino Acid Sequence, Binding Sites, Crystallization, Crystallography, X-Ray, Databases, Protein, Gram-Negative Bacterial Infections microbiology, Humans, Models, Molecular, Protein Conformation, Sequence Alignment, Bacterial Proteins chemistry, Phosphate-Binding Proteins chemistry, Stenotrophomonas maltophilia chemistry

Abstract

During efforts to crystallize the enzyme 2,4-dihydroxyacetophenone dioxygenase (DAD) from Alcaligenes sp. 4HAP, a small number of strongly diffracting protein crystals were obtained after two years of crystal growth in one condition. The crystals diffracted synchrotron radiation to almost 1.0 Å resolution and were, until recently, assumed to be formed by the DAD protein. However, when another crystal form of this enzyme was eventually solved at lower resolution, molecular replacement using this new structure as the search model did not give a convincing solution with the original atomic resolution data set. Hence, it was considered that these crystals might have arisen from a protein impurity, although molecular replacement using the structures of common crystallization contaminants as search models again failed. A script to perform molecular replacement using MOLREP in which the first chain of every structure in the PDB was used as a search model was run on a multi-core cluster. This identified a number of prokaryotic phosphate-binding proteins as scoring highly in the MOLREP peak lists. Calculation of an electron-density map at 1.1 Å resolution based on the solution obtained with PDB entry 2q9t allowed most of the amino acids to be identified visually and built into the model. A BLAST search then indicated that the molecule was most probably a phosphate-binding protein from Stenotrophomonas maltophilia (UniProt ID B4SL31; gene ID Smal_2208), and fitting of the corresponding sequence to the atomic resolution map fully corroborated this. Proteins in this family have been linked to the virulence of antibiotic-resistant strains of pathogenic bacteria and with biofilm formation. The structure of the S. maltophilia protein has been refined to an R factor of 10.15% and an Rfree of 12.46% at 1.1 Å resolution. The molecule adopts the type II periplasmic binding protein (PBP) fold with a number of extensively elaborated loop regions. A fully dehydrated phosphate anion is bound tightly between the two domains of the protein and interacts with conserved residues and a number of helix dipoles.

Published

2016

3. Optimizing modulation transfer spectroscopy signals for frequency locking in the presence of depleted saturating fields.

Author

Hopper DJ and Jaatinen E

Abstract

A theoretical model of modulation transfer spectroscopy (MTS) that includes pump beam depletion is presented and experimentally verified with data covering visible iodine transitions at 532, 543, and 612 nm. This model is used to determine the values for pressure, interaction length, and saturation intensity that yield maximum MTS signals for frequency locking to iodine transitions. The approach is demonstrated for iodine transitions at 532, 633, and 778 nm, with the results showing that theoretically the frequency instability scales inversely to the absorption coefficient.

Published

2008

4. Export of a heterologous cytochrome P450 (CYP105D1) in Escherichia coli is associated with periplasmic accumulation of uroporphyrin.

Author

Akhtar MK, Kaderbhai NN, Hopper DJ, Kelly SL, and Kaderbhai MA

Subjects

Aminolevulinic Acid metabolism, Cytochrome P-450 Enzyme System chemistry, Cytochromes b5 metabolism, Cytoplasm metabolism, DNA metabolism, Dose-Response Relationship, Drug, Escherichia coli metabolism, Heme chemistry, Humans, Hydrogen-Ion Concentration, Models, Biological, Oxygen metabolism, Porphyrins metabolism, Spectrophotometry, Streptomyces griseus enzymology, Cytochrome P-450 Enzyme System metabolism, Escherichia coli enzymology, Periplasm metabolism, Uroporphyrins metabolism

Abstract

This report suggests an important physiological role of a CYP in the accumulation of uroporphyrin I arising from catalytic oxidative conversion of uroporphyrinogen I to uroporphyrin I in the periplasm of Escherichia coli cultured in the presence of 5-aminolevulinic acid. A structurally competent Streptomyces griseus CYP105D1 was expressed as an engineered, exportable form in aerobically grown E. coli. Its progressive induction in the presence of 5-aminolevulinic acid-supplemented medium was accompanied by an accumulation of a greater than 100-fold higher amount of uroporphyrin I in the periplasm relative to cells lacking CYP105D1. Expression of a cytoplasm-resident engineered CYP105D1 at a comparative level to the secreted form was far less effective in promoting porphyrin accumulation in the periplasm. Expression at a 10-fold molar excess over the exported CYP105D1 of another periplasmically exported hemoprotein, the globular core of cytochrome b5, did not substitute the role of the periplasmically localized CYP105D1 in promoting porphyrin production. This, therefore, eliminated the possibility that uroporphyrin accumulation is merely a result of increased hemoprotein synthesis. Moreover, in the strain that secreted CYP105D1, uroporphyrin production was considerably reduced by azole-based P450 inhibitors. Production of both holo-CYP105D1 and uroporphyrin was dependent upon 5-aminolevulinic acid, except that at higher concentrations this resulted in a decrease in uroporphyrin. This study suggests that the exported CYP105D1 oxidatively catalyzes periplasmic conversion of uroporphyrinogen I to uroporphyrin I in E. coli. The findings have significant implications in the ontogenesis of human uroporphyria-related diseases.

Published

2003

5. A cytochrome c from a lupanine-transforming Pseudomonas putida strain is expressed in Escherichia coli during aerobic cultivation and efficiently exported and assembled in the periplasm.

Author

Kaderbhai MA, Hopper DJ, Akhtar KM, Abbas SK, and Kaderbhai NN

Subjects

Aerobiosis, Amino Acid Sequence, Base Sequence, Cloning, Molecular, Cytochrome c Group chemistry, Cytochrome c Group genetics, Cytochrome c Group isolation & purification, Molecular Sequence Data, Protein Transport, Recombinant Proteins metabolism, Sparteine analogs & derivatives, Alkaloids metabolism, Bacterial Proteins metabolism, Cytochrome c Group metabolism, Escherichia coli genetics, Periplasm enzymology, Pseudomonas putida enzymology

Abstract

We have cloned, sequenced, and heterologously expressed a periplasmic cytochrome c from a lupanine-utilizing Pseudomonas putida strain. Aerobic batch cultivation of Escherichia coli TB1 harboring the cytochrome c gene placed downstream of the lac promoter in pUC9 vector resulted in significant production of the holo-cytochrome c in the periplasm ( approximately 4 mg of hemoprotein/liter of culture). The recombinant cytochrome c was purified to homogeneity and was found to be functional in accepting electrons from lupanine hydroxylase while catalyzing hydroxylation of lupanine. Comparison of the N-terminal amino acid sequence of the isolated cytochrome c with that deduced from the DNA sequence indicated that the signal sequence was processed at the bond position predicted by the SigPep program. The molecular size of the cytochrome c determined by electrospray mass spectrometry (9,595) was in precise agreement with that predicted from the nucleotide sequence.

Published

2003

6. Alkylphenol biotransformations catalyzed by 4-ethylphenol methylenehydroxylase.

Author

Hopper DJ and Cottrell L

Subjects

Gas Chromatography-Mass Spectrometry, Phenols chemistry, Stereoisomerism, Substrate Specificity, Mixed Function Oxygenases metabolism, Phenols metabolism, Pseudomonas putida enzymology

Abstract

4-ethylphenol methylenehydroxylase from Pseudomonas putida JD1 acts by dehydrogenation of its substrate to give a quinone methide, which is then hydrated to an alcohol. It was shown to be active with a range of 4-alkylphenols as substrates. 4-n-propylphenol, 4-n-butylphenol, chavicol, and 4-hydroxydiphenylmethane were hydroxylated on the methylene group next to the benzene ring and produced the corresponding chiral alcohol as the major product. The alcohols 1-(4'-hydroxyphenyl)propanol and 1-(4'-hydroxyphenyl)-2-propen-1-ol, produced by the biotransformation of 4-n-propylphenol and chavicol, respectively, were shown to be R(+) enantiomers. 5-Indanol, 6-hydroxytetralin, 4-isopropylphenol, and cyclohexylphenol, with cyclic or branched alkyl groups, gave the corresponding vinyl compounds as their major products.

Published

2003

7. The quinohaemoprotein lupanine hydroxylase from Pseudomonas putida.

Author

Hopper DJ and Kaderbhai MA

Subjects

Amino Acid Sequence, Cloning, Molecular, Molecular Sequence Data, Oxidoreductases Acting on CH-NH Group Donors chemistry, PQQ Cofactor, Quinolones chemistry, Quinones chemistry, Recombinant Proteins biosynthesis, Bacterial Proteins genetics, Oxidoreductases Acting on CH-NH Group Donors genetics, Pseudomonas putida enzymology

Abstract

Lupanine hydroxylase catalyses the first reaction in the catabolism of the alkaloid lupanine by Pseudomonas putida. It dehydrogenates the substrate, which can then be hydrated. It is a monomeric protein of M(r) 72,000 and contains a covalently bound haem and a molecule of PQQ. The gene for this enzyme has been cloned and sequenced and the derived protein sequence has a 26 amino acid signal sequence at the N-terminal for translocation of the protein to the periplasm. Many of the features seen in the sequence of lupanine hydroxylase are common with other quinoproteins including the W-motifs that are characteristic of the eight-bladed propeller structure of methanol dehydrogenase. However, the unusual disulfide bridge between adjacent cysteines that is present in some PQQ-containing enzymes is absent in lupanine hydroxylase. The C-terminal domain contains characteristics of a cytochrome c and overall the sequence shows similarities with that of the quinohaemoprotein, alcohol dehydrogenase from Comamonas testosteroni. The gene coding for lupanine hydroxylase has been successfully expressed in Escherichia coli and a procedure has been developed to renature and reactivate the enzyme, which was found to be associated with the inclusion bodies. Reactivation required addition of PQQ and was dependent on calcium ions.

Published

2003

8. Cloning, sequencing and heterologous expression of the gene for lupanine hydroxylase, a quinocytochrome c from a Pseudomonas sp.

Author

Hopper DJ, Kaderbhai MA, Marriott SA, Young M, and Rogozinski J

Subjects

Amino Acid Sequence, Base Sequence, Binding Sites, Calcium metabolism, Cloning, Molecular, Escherichia coli genetics, Gene Expression Regulation, Bacterial, Molecular Sequence Data, PQQ Cofactor, Protein Sorting Signals, Protein Transport, Quinolones chemistry, Quinolones metabolism, Quinones chemistry, Quinones metabolism, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Restriction Mapping, Sequence Analysis, Sequence Homology, Amino Acid, Oxidoreductases Acting on CH-NH Group Donors genetics, Oxidoreductases Acting on CH-NH Group Donors metabolism, Pseudomonas genetics

Abstract

The gene encoding the enzyme lupanine hydroxylase was isolated by PCR using chromosomal DNA from a lupanine-utilizing Pseudomonas sp. as template and primers based on the sequences of the N- and C-termini of the purified protein. The derived sequence for the mature gene product gave a protein with an M (r) of 72256, in good agreement with the value found by SDS/PAGE of the pure enzyme, and contained the sequences of several peptides obtained after endoproteinase Lys-C digestion of the pure enzyme. The gene, under the transcriptional control of a phoA promotor and with the Escherichia coli alkaline phosphatase signal sequence, was expressed in E. coli containing a plasmid expressing the genes for cytochrome c maturation proteins constitutively. Haem-containing inactive protein in inclusion bodies was renatured and reactivated with pyrroloquinoline quinone (PQQ) and Ca(2+) to give active enzyme. The lupanine hydroxylase (luh) gene coded for a protein with a cleavable 26-residue signal sequence at its N-terminus, required for the transport of the enzyme to its periplasmic location. Analysis of the protein sequence showed that it contains two domains, a large PQQ-binding N-terminal domain and a smaller cytochrome c C-terminal domain. Comparison of the derived sequence with those of other proteins showed considerable similarity with other quino(haemo)proteins, including alcohol dehydrogenases from a variety of bacteria. The PQQ-binding domain sequence contains W motifs, characteristic of the eight-bladed "propeller" structure of methanol dehydrogenase, but lacks the unusual disulphide ring structure formed from two adjacent cysteines seen in this enzyme. The C-terminus shares some similarity with bacterial cytochrome c and includes the haem-binding consensus sequence CXXCH.

Published

2002