Otzen_2007_Biochim.Biophys.Acta_1774_323

Reference

Title : Aggregation as the basis for complex behaviour of cutinase in different denaturants - Otzen_2007_Biochim.Biophys.Acta_1774_323
Author(s) : Otzen DE , Giehm L , Baptista RP , Kristensen SR , Melo EP , Pedersen S
Ref : Biochimica & Biophysica Acta , 1774 :323 , 2007
Abstract :

We have previously described the complexity of the folding of the lipolytic enzyme cutinase from F. solani pisi in guanidinium chloride. Here we extend the refolding analysis by refolding from the pH-denatured state and analyze the folding behaviour in the presence of the weaker denaturant urea and the stronger denaturant guanidinium thiocyanate. In urea there is excellent consistency between equilibrium and kinetic data, and the intermediate accumulating at low denaturant concentrations is off-pathway. However, in GdmCl, refolding rates, and consequently the stability of the native state, vary significantly depending on whether refolding takes place from the pH- or GdmCl-denatured state, possibly due to transient formation of aggregates during folding from the GdmCl-denatured state. In GdmSCN, stability is reduced by several kcal/mol with significant aggregation in the unfolding transition region. The basis for the large variation in folding behaviour may be the denaturants' differential ability to support formation of exposed hydrophobic regions and consequent changes in aggregative properties during refolding.

PubMedSearch : Otzen_2007_Biochim.Biophys.Acta_1774_323
PubMedID: 17208524

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Citations formats

Otzen DE, Giehm L, Baptista RP, Kristensen SR, Melo EP, Pedersen S (2007)
Aggregation as the basis for complex behaviour of cutinase in different denaturants
Biochimica & Biophysica Acta 1774 :323

Otzen DE, Giehm L, Baptista RP, Kristensen SR, Melo EP, Pedersen S (2007)
Biochimica & Biophysica Acta 1774 :323