| Literature DB >> 26239214 |
Arne Schön1, Benjamin R Clarkson1, Rogelio Siles1, Patrick Ross2, Richard K Brown2, Ernesto Freire3.
Abstract
Protein aggregation is a major issue affecting the long-term stability of protein preparations. Proteins exist in equilibrium between the native and denatured or partially denatured conformations. Often denatured or partially denatured conformations are prone to aggregate because they expose to solvent the hydrophobic core of the protein. The aggregation of denatured protein gradually shifts the protein equilibrium toward increasing amounts of denatured and ultimately aggregated protein. Recognizing and quantitating the presence of denatured protein and its aggregation at the earliest possible time will bring enormous benefits to the identification and selection of optimal solvent conditions or the engineering of proteins with the best stability/aggregation profile. In this article, a new approach that allows simultaneous determination of structural stability and the amount of denatured and aggregated protein is presented. This approach is based on the analysis of the concentration dependence of the Gibbs energy (ΔG) of protein stability. It is shown that three important quantities can be evaluated simultaneously: (i) the population of denatured protein, (ii) the population of aggregated protein, and (iii) the fraction of denatured protein that is aggregated.Entities:
Keywords: Denatured state aggregation; Isothermal chemical denaturation; Protein conformational equilibrium; Thermodynamic linkage equilibrium and aggregation
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Year: 2015 PMID: 26239214 DOI: 10.1016/j.ab.2015.07.013
Source DB: PubMed Journal: Anal Biochem ISSN: 0003-2697 Impact factor: 3.365