Protein Folding Intermediates: Native-State Hydrogen Exchange

14 July 1995

journal article
Published by American Association for the Advancement of Science (AAAS) in Science

Vol. 269 (5221), 192-197
https://doi.org/10.1126/science.7618079

Abstract

The hydrogen exchange behavior of native cytochrome c in low concentrations of denaturant reveals a sequence of metastable, partially unfolded forms that occupy free energy levels reaching up to the fully unfolded state. The step from one form to another is accomplished by the unfolding of one or more cooperative units of structure. The cooperative units are entire omega loops or mutually stabilizing pairs of whole helices and loops. The partially unfolded forms detected by hydrogen exchange appear to represent the major intermediates in the reversible, dynamic unfolding reactions that occur even at native conditions and thus may define the major pathway for cytochrome c folding.

Keywords

This publication has 43 references indexed in Scilit:

How does a protein fold?
Nature, 1994
Kinetic and equilibrium intermediates in protein folding
Protein Engineering, Design and Selection, 1994
A noncovalent peptide complex as a model for an early folding intermediate of cytochrome c
Biochemistry, 1993
Protein internal flexibility and global stability: Effect of urea on hydrogen exchange rates of bovine pancreatic trypsin inhibitor
Biochemistry, 1993
Residual helical structure in the C-terminal fragment of cytochrome c
Biochemistry, 1993
Protein interactions with urea and guanidinium chloride
Journal of Molecular Biology, 1992
Stable submolecular folding units in a non-compact form of cytochrome c
Journal of Molecular Biology, 1991
High-resolution three-dimensional structure of horse heart cytochrome c
Journal of Molecular Biology, 1990
Proton resonance assignments of horse ferrocytochrome c
Biochemistry, 1989
Conformation change of cytochrome c
Journal of Molecular Biology, 1981

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