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Research Article

Lower kinetic limit to protein thermal stability: A proposal regarding protein stability in vivo and its relation with misfolding diseases

  1. Isabel M. Plaza del Pino,
  2. Beatriz Ibarra-Molero,
  3. Jose M. Sanchez-Ruiz*

Article first published online: 11 MAY 2000

DOI: 10.1002/(SICI)1097-0134(20000701)40:1<58::AID-PROT80>3.0.CO;2-M

Issue

Proteins: Structure, Function, and Bioinformatics

Proteins: Structure, Function, and Bioinformatics

Volume 40, Issue 1, pages 58–70, 1 July 2000

Additional Information

How to Cite

Plaza del Pino, I. M., Ibarra-Molero, B. and Sanchez-Ruiz, J. M. (2000), Lower kinetic limit to protein thermal stability: A proposal regarding protein stability in vivo and its relation with misfolding diseases. Proteins, 40: 58–70. doi: 10.1002/(SICI)1097-0134(20000701)40:1<58::AID-PROT80>3.0.CO;2-M

Author Information

  1. Facultad de Ciencias, Departamento de Quimica Fisica, Universidad de Granada, Granada, Spain

  1. Department of Chemistry, Penn State University, University Park, Pennsylvania

*Departamento de Quimica Fisica. Fuentenueva s/n. 18071-Granada, Spain

Publication History

  1. Issue published online: 11 MAY 2000
  2. Article first published online: 11 MAY 2000
  3. Manuscript Accepted: 10 FEB 2000
  4. Manuscript Received: 8 NOV 1999

Funded by

  • DGES (Spanish Ministry of Education and Culture). Grant Number: PB96-1439

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Keywords:

  • denaturation;
  • irreversibility;
  • energetics;
  • thermophilic proteins;
  • amyloids

Abstract

In vitro thermal denaturation experiments suggest that, because of the possibility of irreversible alterations, thermodynamic stability (i.e., a positive value for the unfolding Gibbs energy) does not guarantee that a protein will remain in the native state during a given timescale. Furthermore, irreversible alterations are more likely to occur in vivo than in vitro because (a) some irreversible processes (e.g., aggregation, “undesirable” interactions with other macromolecular components, and proteolysis) are expected to be fast in the “crowded” cellular environment and (b) in many cases, the relevant timescale in vivo (probably related to the half-life for protein degradation) is expected to be longer than the timescale of the usual in vitro experiments (of the order of minutes). We propose, therefore, that many proteins (in particular, thermophilic proteins and “complex” proteins systems) are designed (by evolution) to have significant kinetic stability when confronted with the destabilizing effect of irreversible alterations. We show that, as long as these alterations occur mainly from non-native states (a Lumry-Eyring scenario), the required kinetic stability may be achieved through the design of a sufficiently high activation barrier for unfolding, which we define as the Gibbs energy barrier that separates the native state from the non-native ensemble (unfolded, partially folded, and misfolded states) in the following generalized Lumry-Eyring model:

  • equation image

Finally, using familial amyloid polyneuropathy (FAP) as an illustrative example, we discuss the relation between stability and amyloid fibril formation in terms of the above viewpoint, which leads us to the two following tentative suggestions: (a) the hot spot defined by the FAP-associated amyloidogenic mutations of transthyretin reflects the structure of the transition state for unfolding and (b) substances that decrease the in vitro rate of transthyretin unfolding could also be inhibitors of amyloid fibril formation. Proteins 2000;40:58–70. © 2000 Wiley-Liss, Inc.

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