Your search keyword '"Creaser, P"' showing total 12 results

1. A novel manual method for protein-sequence analysis

Author

Chang, J Y and Creaser, E H

Abstract

A novel manual method for protein-sequence analysis is described. Three peptides, the hexapeptide (Leu-TRP-Met-Arg-Phe-Ala), insulin A chain and glucagon were used to test this technique. Peptides (1 or 2 nmol) were hydrolysed with acid and their qualitative amino acid compositions were confirmed by reacting with 4-NN-dimethylaminoazobenzene-4'-sulphonylchloride and 4-NN-dimethylaminoazobenzene 4'-isothiocyanate. Sequence determination of 20-200 nmol of peptide was then performed by the combined use of phenyl isothiocyanate and 4-NN-dimethylaminoazobenzene 4'-isothiocyanate, a new procedure that is analogous to the dansyl-Edman method with the replacement of dansyl chloride by 4-NN-dimethylaminoazobenzene 4'-isothiocyanate as the N-terminal residue determination reagent. On t.l.c. this new N-terminal reagent gave brightly coloured 4-NN-dimethylaminoazobenzene-4-thiohydantoins of amino acids and showed the following advantages: (1) the detection sensitivity is in the pmol range; (2) u.v. observation is not required; (3) there is no destruction of acid-labile amino acids; (4) two-dimensional t.l.c. separation is adequate to identify 24 amino acids, except leucine and isoleucine (this pair of amino acids can be resolved by using 4-NN-dimethylaminoazobenzene-4'-sulphonyl chloride); (5) the determination of a new N-terminal residue (from coupling to t.l.c. identification) takes only 3 h; (6) the colour difference beteen isothiocyanate, thiocarbamoyl and thiohydantoin derivatives facilitates the identifications.

Published

1976

2. Purification and preliminary characterization of alcohol dehydrogenase from Aspergillus nidulans

Author

Creaser, E H, Porter, R L, Britt, K A, Pateman, J A, and Doy, C H

Abstract

Aspergillus alcohol dehydrogenase is produced in response to growth in the presence of a wide variety of inducers, of which the most effective are short-chain alcohols and ketones, e.g. butan-2-one and propan-2-ol. The enzyme can be readily extracted from fresh or freeze-dried cells and purified to homogeneity on Blue Sepharose in a single step by using specific elution with NAD+ and pyrazole. The pure enzyme has Mr 290 000 by electrophoresis or gel filtration; it is a homopolymer with subunit Mr 37 500 by electrophoresis in sodium dodecyl sulphate; its amino acid composition corresponds to Mr 37 900, and the native enzyme contains one zinc atom per subunit. The enzyme is NAD-specific and has a wide substrate activity in the forward and reverse reactions; its activity profile is not identical with those of other alcohol dehydrogenases.

Published

1985

3. Purification and properties of histidinol dehydrogenases from psychrophilic, mesophilic and thermophilic bacilli

Author

Lindsay, J A and Creaser, E H

Abstract

As a first step in elucidating one molecular mechanism of adaptation to life at extreme temperatures, we purified and characterized the enzyme histidinol dehydrogenase (EC 1.1.1.23) from a number of bacilli whose growth temperatures range from 5 degrees t to 90 degrees C. The enzymes were purified by (NH4)2SO4 precipitation, ion-exchange chromatography on Sephadex, affinity chromatography on histamine- or histidine-Sepharose and preparative gradient gel electrophoresis. All had similar mol.wts. (29200), sedimentation coefficients (S20,w 2.56S), affinities for histidinol and NAD+ (Km = 48 micron and 0.2 mM respectively) and all had pH optima at 9.6. Marked differences were observed in stability with respect to temperature and the temperature at which the initial velocity for histidinol dehydrogenation was optimal. These optima range from 25 degrees C for the enzyme from the psychrophilic species through to 41 degrees C for the mesophiles to 85-92 degrees C for the extreme thermophiles. It is concluded that the ability of the enzymes to operate at their various optimum temperatures is an intrinsic property of their amino acid sequences.

Published

1977

4. 4-NN-dimethylaminoazobenzene 4′-isothiocyanate, a new chromophoric reagent for protein sequence analysis

Author

Chang, J Y, Creaser, E H, and Bentley, K W

Abstract

4-NN-Dimethylaminoazobenzene 4‘-isothiocyanate was synthesized for the purpose of improving the ease and sensitivity of peptide sequence analysis. The method of 4-NN-dimethylaminoazobenzene 4′-isothiocyanate synthesis, the preparation of 24 4-NN-dimethylaminoazobenzene-4′-thiohydantoins of amino acids and their t.l.c. separation are described. All the thiohydantoins, except those of leucine and isoleucine, could be satisfactorily separated by chromatography on a two-dimensional polyamide sheet. The sensitive azo group permits the detection of 4-NN-dimethylaminoazobenzene-4′-thiohydantoins of amino acids as red spots down to pmol amounts directly on the sheet. A simple sensitive method for sequencing dipeptides and the first two or three N-terminal amino acids of proteins is also reported. The colour change of the spots from purple to blue to red after being exposed to HCl vapour, corresponding to the chemical change from 4-NN-dimethylaminoazobenzene-4′ ’ isothiocyanate to the 4-NN-dimethylaminoazobenzene-4′-thiocarbamoyl amino acid derivative to the 4-NN-dimethylaminoazobenzene-4′-thiohydantoin amino acid derivative, reveals a very interesting and valuable feature of this reagent.

Published

1976

5. Amino acid substitutions in mutant forms of histidinol dehydrogenase from Neurospora crassa

Author

Bennett, D J and Creaser, E H

Abstract

Amino acid changes in the enzyme l-histidinol dehydrogenase (l-histidinol–NAD oxidoreductase, EC 1.1.1.23) have been determined between the wild-type Neurospora crassa and two temperature-sensitive mutants. Comparison was made between amino acid analyses of peptides of differing electrophoretic and chromatographic mobilities resulting from tryptic and chymotryptic digestion of protein from wild-type and mutant K26, and wild-type and mutant K445 strains, respectively. The analyses demonstrate the substitution of aspartic acid for alanine in mutant K26, and leucine for histidine in mutant K445. The effects of the resulting changes in polarity and charge are discussed in relation to the catalytic functioning of the proteins.

Published

1967

6. The purification and properties of histidinol dehydrogenase from Neurospora crassa

Author

Creaser, EH, Bennett, DJ, and Drysdale, RB

Published

1967

7. The assimilation of amino acids by bacteria. 22. The effect of 8-azaguanine upon enzyme formation in Staphylococcus aureus

Author

Creaser, E. H.

Published

1956

8. A comparison of the nucleic acids of rat liver and Novikoff hepatoma

Author

Creaser, E H and Spencer, J. H.

Published

1960

9. Purification of a trifunctional enzyme, catalysing three steps of the histidine pathway, from Neurospora crassa

Author

Minson, A. C. and Creaser, E H

Abstract

1. A procedure is described for the purification of an enzyme from Neurospora crassa that has three catalytic functions. These are 1-N-(5′-phosphoribosyl)-ATP pyrophosphohydrolase, 1-N-(5′-phosphoribosyl)-AMP cyclohydrolase and histidinol dehydrogenase (l-histidinol–NAD oxidoreductase, EC 1.1.1.23), and are responsible for the catalysis of reactions 2, 3 and 10 in the histidine pathway. The ratio of these three catalytic activities remains approximately the same throughout the purification procedure. Evidence is presented that the purified preparations contain a single protein exhibiting association–dissociation equilibria.

Published

1969

10. Qualitative determination of N-terminal amino acids of peptides and proteins with cobalt(III) chelates

Author

Bentley, Keith W. and Creaser, Ernest H.

Abstract

1. A method of N-terminal peptide-bond hydrolysis with the cis-β-hydroxyaquo(triethylenetetramine)cobalt(III) ion, i.e. β-[Co(trien)(OH)(OH2)]2+, is reported. The method has been demonstrated with 22 small peptides and ten proteins. 2. The procedure is rapid (an N-terminal amino acid determination can be made easily in one day), it involves no acid hydrolysis step and thus no destruction of labile amino acids, and it involves the use of easily prepared inexpensive reagents. 3. The released N-terminal amino acids can be identified as their cobalt(III) derivatives, or directly as the amino acid or as their dansylated derivatives. 4. The method is to treat 1 μmol of peptide or protein with β-[Co(trien)(OH)(OH2)]2+ reagent at pH8.0, 45°C for 3h. Addition of 0.5m-phosphate buffer, pH10.5 at 45°C for 10min cleaves the N-terminal bidentate amino acid–cobalt complex, which can be identified directly. For greater sensitivity with 10nmol of peptide) the free amino acid is prepared from the complex by treatment (with NaCN (0.1m, 40°C, 30min), or H2S or NaBH4 (25°C, 5min), dried, dansylated and the dansyl-amino acid identified by high-voltage electrophoresis. The method is unaffected by the presence of 4–8m-urea, but will not cleave blocked N-terminal acids.

Published

1973

11. C-terminal analysis of histidinol dehydrogenase from Neurospora crassa

Author

Bennett, D J, Creaser, E H, and MacDonald, P W

Published

1968

12. Further characterization of a protein promoting aggregation of retina cells

Author

Creaser, E H and Russell, L M

Published

1971