Chemical chaperone-mediated protein folding: stabilization of P22 tailspike folding intermediates by glycerol
Glycerol
Protein Denaturation
Protein Folding
0303 health sciences
Glycoside Hydrolases
Temperature
Viral Tail Proteins
Kinetics
Protein Subunits
03 medical and health sciences
Spectrometry, Fluorescence
Solvents
Thermodynamics
Urea
Institut für Biochemie und Biologie
Bacteriophage P22
DOI:
10.1515/bc.2007.096
Publication Date:
2007-07-27T13:56:06Z
AUTHORS (3)
ABSTRACT
Abstract
Polyol co-solvents such as glycerol increase the thermal stability of proteins. This has been explained by preferential hydration favoring the more compact native over the denatured state. Although polyols are also expected to favor aggregation by the same mechanism, they have been found to increase the folding yields of some large, aggregation-prone proteins. We have used the homotrimeric phage P22 tailspike protein to investigate the origin of this effect. The folding of this protein is temperature-sensitive and limited by the stability of monomeric folding intermediates. At non-permissive temperature (≥35°C), tailspike refolding yields were increased significantly in the presence of 1–4 m glycerol. At low temperature, tailspike refolding is prevented when folding intermediates are destabilized by the addition of urea. Glycerol could offset the urea effect, suggesting that the polyol acts by stabilizing crucial folding intermediates and not by increasing solvent viscosity. The stabilization effect of glycerol on tailspike folding intermediates was confirmed in experiments using a temperature-sensitive folding mutant protein, by fluorescence measurements of subunit folding kinetics, and by temperature up-shift experiments. Our results suggest that the chemical chaperone effect of polyols observed in the folding of large proteins is due to preferential hydration favoring structure formation in folding intermediates.
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