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Literature DB >> 4776867

Refolding of triose phosphate isomerase.

Abstract

The refolding and reactivation of the glycolytic enzyme triose phosphate isomerase (EC 5.3.1.1) has been studied. The enzyme, which is a dimer, is disaggregated and unfolded in solutions of guanidinium chloride. Unfolding, followed by changes in E(233), took place quite rapidly in 3m-guanidinium chloride (i.e. with a half-life of about 1 min). Refolding also took place rapidly when the solution was diluted about tenfold; two first-order processes could be resolved. Regain of enzymic activity was followed by diluting the solution of the denatured enzyme in guanidinium chloride into assay mixture. The half-life (i.e. the time when the activity was half the final activity) depended markedly on the concentration of protein at low concentrations (about 100ng/ml), but at higher concentrations the half-life became independent of concentration. Thus at low concentrations dimerization was a rate-determining step and this is taken to indicate that the monomers showed little or no activity under these conditions. The rate of regain of enzymic activity was the same as the rate of the slower process of refolding, which was detected spectroscopically. The native enzyme was resistant to proteolysis; high concentrations of subtilisin prevented regain of activity, but at lower concentrations refolding competed with proteolysis.

Entities: Chemical

Mesh：

Substances：

Year: 1973 PMID： 4776867 PMCID： PMC1165801 DOI： 10.1042/bj1350165

Source DB: PubMed Journal: Biochem J ISSN： 0264-6021 Impact factor: 3.857

20 in total

1. The assembly pathway of lactic dehydrogenase isozymes from their unfolded subunits.

Authors: A Levitzki
Journal: FEBS Lett Date: 1972-08-15 Impact factor: 4.124

2. THE EFFECT OF COMPOUNDS OF THE UREA-GUANIDINIUM CLASS ON THE ACTIVITY COEFFICIENT OF ACETYLTETRAGLYCINE ETHYL ESTER AND RELATED COMPOUNDS.

Authors: D R ROBINSON; W P JENCKS
Journal: J Am Chem Soc Date: 1965-06-05 Impact factor: 15.419

Review 3. DNA-protein interactions.

Authors: P H Von Hippel; J D McGhee
Journal: Annu Rev Biochem Date: 1972 Impact factor: 23.643

4. Kinetics of unfolding and refolding of proteins. 3. Results for lysozyme.

Authors: C Tanford; K C Aune; A Ikai
Journal: J Mol Biol Date: 1973-01-10 Impact factor: 5.469

5. Equilibrium and kinetic studies on the reversible dissociation of yeast enolase by neutral salts.

Authors: T H Gawronski; E W Westhead
Journal: Biochemistry Date: 1969-11 Impact factor: 3.162

6. In vitro assembly of aldolase. Kinetics of refolding, subunit reassociation, and reactivation.

Authors: J W Teipel
Journal: Biochemistry Date: 1972-10-24 Impact factor: 3.162

7. Kinetics of unfolding and refolding of proteins. I. Mathematical analysis.

Authors: A Ikai; C Tanford
Journal: J Mol Biol Date: 1973-01-10 Impact factor: 5.469

8. The reaction of 2,4,6-trinitrobenzenesulphonic acid with amino acids, Peptides and proteins.

Authors: R B Freedman; G K Radda
Journal: Biochem J Date: 1968-07 Impact factor: 3.857

9. Matrix-bound protein subunits.

Authors: W W Chan
Journal: Biochem Biophys Res Commun Date: 1970-12-09 Impact factor: 3.575

10. Dissociation of yeast enolase into active monomers.

Authors: S Keresztes-Nagy; R Orman
Journal: Biochemistry Date: 1971-06-22 Impact factor: 3.162

17 in total

1. Thermodynamic characterization of yeast triosephosphate isomerase refolding: insights into the interplay between function and stability as reasons for the oligomeric nature of the enzyme.

Authors: Hugo Nájera; Miguel Costas; D Alejandro Fernández-Velasco
Journal: Biochem J Date: 2003-03-15 Impact factor: 3.857

Refolding of triose phosphate isomerase.

1. The assembly pathway of lactic dehydrogenase isozymes from their unfolded subunits.

2. THE EFFECT OF COMPOUNDS OF THE UREA-GUANIDINIUM CLASS ON THE ACTIVITY COEFFICIENT OF ACETYLTETRAGLYCINE ETHYL ESTER AND RELATED COMPOUNDS.

Review 3. DNA-protein interactions.

4. Kinetics of unfolding and refolding of proteins. 3. Results for lysozyme.

5. Equilibrium and kinetic studies on the reversible dissociation of yeast enolase by neutral salts.

6. In vitro assembly of aldolase. Kinetics of refolding, subunit reassociation, and reactivation.

7. Kinetics of unfolding and refolding of proteins. I. Mathematical analysis.

8. The reaction of 2,4,6-trinitrobenzenesulphonic acid with amino acids, Peptides and proteins.

9. Matrix-bound protein subunits.

10. Dissociation of yeast enolase into active monomers.

1. Thermodynamic characterization of yeast triosephosphate isomerase refolding: insights into the interplay between function and stability as reasons for the oligomeric nature of the enzyme.

2. An intersubunit lock-and-key 'clasp' motif in the dimer interface of Delta class glutathione transferase.

3. In search of new lead compounds for trypanosomiasis drug design: a protein structure-based linked-fragment approach.

4. Long-lived conformational isomerism of protein dimers: the role of the free energy of subunit association.

5. Focused functional dynamics of supramolecules by use of a mixed-resolution elastic network model.

6. Reactivation of triosephosphate isomerase from three trypanosomatids and human: effect of suramin.

7. Studies of triose phosphate isomerase by hydrogen exchange.

8. Control of oligomeric enzyme thermostability by protein engineering.

9. Design, creation, and characterization of a stable, monomeric triosephosphate isomerase.

10. Phosphonomethyl analogues of phosphate ester glycolytic intermediates.