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Literature DB >> 9232646

Absence of a stable intermediate on the folding pathway of protein A.

Y Bai¹, A Karimi, H J Dyson, P E Wright.

Abstract

The B-domain of protein A has one of the simplest protein topologies, a three-helix bundle. Its folding has been studied as a model for elementary steps in the folding of larger proteins. Earlier studies suggested that folding might occur by way of a helical hairpin intermediate. Equilibrium hydrogen exchange measurements indicate that the C-terminal helical hairpin could be a potential folding intermediate. Kinetic refolding experiments were performed using stopped-flow circular dichroism and NMR hydrogen-deuterium exchange pulse labeling. Folding of the entire molecule is essentially complete within the 6 ms dead time of the quench-flow apparatus, indicating that the intermediate, if formed, progresses rapidly to the final folded state. Site-directed mutagenesis of the isoleucine residue at position 16 was used to generate a variant protein containing tryptophan (the 116 W mutant). The formation of the putative folding intermediate was expected to be favored in this mutant at the expense of the native folded form, due to predicted unfavorable steric interactions of the bulky tryptophan side chain in the folded state. The 116 W mutant refolds completely within the dead time of a stopped-flow fluorescence experiment. No partly folded intermediate could be detected by either kinetic or equilibrium measurements. Studies of peptide fragments suggest that the protein A sequence has an intrinsic propensity to form a helix II/helix III hairpin. However, its stability appears to be marginal (of the order of 1/2 kT) and it could not be an obligatory intermediate on a defined folding pathway. These results explicitly demonstrate that the protein A B domain folds extremely rapidly by an apparent two-state mechanism without formation of stable partly folded intermediates. Similar mechanisms may also be involved in the rapid folding of subdomains of larger proteins to form the compact molten globule intermediates that often accumulate during the folding process.

Entities: Chemical

Mesh：

Substances：

Year: 1997 PMID： 9232646 PMCID： PMC2143746 DOI： 10.1002/pro.5560060709

Source DB: PubMed Journal: Protein Sci ISSN： 0961-8368 Impact factor: 6.725

48 in total

1. In situ neutralization in Boc-chemistry solid phase peptide synthesis. Rapid, high yield assembly of difficult sequences.

Authors: M Schnölzer; P Alewood; A Jones; D Alewood; S B Kent
Journal: Int J Pept Protein Res Date: 1992 Sep-Oct

2. The folding of hen lysozyme involves partially structured intermediates and multiple pathways.

Authors: S E Radford; C M Dobson; P A Evans
Journal: Nature Date: 1992-07-23 Impact factor: 49.962

3. Folding of chymotrypsin inhibitor 2. 1. Evidence for a two-state transition.

Authors: S E Jackson; A R Fersht
Journal: Biochemistry Date: 1991-10-29 Impact factor: 3.162

4. A test of the linear extrapolation of unfolding free energy changes over an extended denaturant concentration range.

Authors: M M Santoro; D W Bolen
Journal: Biochemistry Date: 1992-05-26 Impact factor: 3.162

Review 5. Intermediates in the folding reactions of small proteins.

Authors: P S Kim; R L Baldwin
Journal: Annu Rev Biochem Date: 1990 Impact factor: 23.643

6. Theory of cooperative transitions in protein molecules. I. Why denaturation of globular protein is a first-order phase transition.

Authors: E I Shakhnovich; A V Finkelstein
Journal: Biopolymers Date: 1989-10 Impact factor: 2.505

7. Three-dimensional solution structure of the B domain of staphylococcal protein A: comparisons of the solution and crystal structures.

Authors: H Gouda; H Torigoe; A Saito; M Sato; Y Arata; I Shimada
Journal: Biochemistry Date: 1992-10-13 Impact factor: 3.162

8. Truncated, branched, and/or cyclic analogues of neuropeptide Y: importance of the pancreatic peptide fold in the design of specific Y2 receptor ligands.

Authors: M T Reymond; L Delmas; S C Koerber; M R Brown; J E Rivier
Journal: J Med Chem Date: 1992-10-02 Impact factor: 7.446

9. Folding of peptide fragments comprising the complete sequence of proteins. Models for initiation of protein folding. I. Myohemerythrin.

Authors: H J Dyson; G Merutka; J P Waltho; R A Lerner; P E Wright
Journal: J Mol Biol Date: 1992-08-05 Impact factor: 5.469

10. Folding of peptide fragments comprising the complete sequence of proteins. Models for initiation of protein folding. II. Plastocyanin.

Authors: H J Dyson; J R Sayre; G Merutka; H C Shin; R A Lerner; P E Wright
Journal: J Mol Biol Date: 1992-08-05 Impact factor: 5.469

41 in total

Absence of a stable intermediate on the folding pathway of protein A.

1. In situ neutralization in Boc-chemistry solid phase peptide synthesis. Rapid, high yield assembly of difficult sequences.

2. The folding of hen lysozyme involves partially structured intermediates and multiple pathways.

3. Folding of chymotrypsin inhibitor 2. 1. Evidence for a two-state transition.

4. A test of the linear extrapolation of unfolding free energy changes over an extended denaturant concentration range.

Review 5. Intermediates in the folding reactions of small proteins.

6. Theory of cooperative transitions in protein molecules. I. Why denaturation of globular protein is a first-order phase transition.

7. Three-dimensional solution structure of the B domain of staphylococcal protein A: comparisons of the solution and crystal structures.

8. Truncated, branched, and/or cyclic analogues of neuropeptide Y: importance of the pancreatic peptide fold in the design of specific Y2 receptor ligands.

9. Folding of peptide fragments comprising the complete sequence of proteins. Models for initiation of protein folding. I. Myohemerythrin.

10. Folding of peptide fragments comprising the complete sequence of proteins. Models for initiation of protein folding. II. Plastocyanin.

Review 1. The hydrogen exchange core and protein folding.

2. Staphylococcal protein A: unfolding pathways, unfolded states, and differences between the B and E domains.

3. Exploring the origins of topological frustration: design of a minimally frustrated model of fragment B of protein A.

4. Three-helix-bundle protein in a Ramachandran model.

5. Structure and functional interactions of the Tsg101 UEV domain.

6. A structure-based method for derivation of all-atom potentials for protein folding.

7. Folding a protein in a computer: an atomic description of the folding/unfolding of protein A.

8. The dual role of a loop with low loop contact distance in folding and domain swapping.

9. Dynamics of an ultrafast folding subdomain in the context of a larger protein fold.

10. Kinks, loops, and protein folding, with protein A as an example.