EVIDENCE FOR A 2-STATE TRANSITION IN THE FOLDING PROCESS OF THE ACTIVATION DOMAIN OF HUMAN PROCARBOXYPEPTIDASE-A2

被引：93

作者：

VILLEGAS, V

AZUAGA, A

CATASUS, L

REVERTER, D

MATEO, PL

AVILES, FX

SERRANO, L

机构：

[1] EUROPEAN MOLEC BIOL LAB, D-69012 HEIDELBERG, GERMANY

[2] UNIV AUTONOMA BARCELONA, DEPT BIOQUIM, E-08193 BARCELONA, SPAIN

[3] UNIV AUTONOMA BARCELONA, INST BIOL FONAMENTAL, E-08193 BARCELONA, SPAIN

[4] UNIV GRANADA, FAC CIENCIAS, DEPT QUIM FIS, E-18071 GRANADA, SPAIN

来源：

BIOCHEMISTRY | 1995年 / 34卷 / 46期

关键词：

D O I：

10.1021/bi00046a017

中图分类号：

Q5 [生物化学]; Q7 [分子生物学];

学科分类号：

071010 ; 081704 ;

摘要：

The activation domain of human procarboxypeptidase A2 (ADA2h), a globular open-sandwich alpha + beta domain with 80 residues and no disulfide bridges, has been studied by thermodynamic and kinetic analysis. Equilibrium denaturation by urea or temperature is fully reversible at pH 7.0 and fits to a two-state transition. The Gibbs energy of unfolding extrapolated to null concentration of chemical denaturant, Delta G(H2O), at pH 7.0 and 298 K, is calculated to be 17.0 +/- 1 kJ mol(-1), which is within experimental error of the value determined by differential scanning calorimetry, 15.1 +/- 2 kJ mol(-1). Kinetics of unfolding and refolding followed by fluorescence do not show the presence of any kinetic intermediate accumulating in the folding reaction. A value for Delta G(H2O) of 17.9 +/- 0.7 kJ mol(-1) can be extrapolated from the kinetic data. All these data indicate that the folding pathway of this domain is consistent with a two-state model (with the exception of the cis-Pro intermediates). More importantly, the analysis of this and several other small domains or proteins supports the hypothesis that stable kinetic folding intermediates are not necessary for a protein to fold. There seems to be a relationship between the size of a protein and the presence of stable kinetic intermediates. Globular proteins with less than 80 residues and no disulfide bonds follow a two-state transition, while proteins larger than 100 residues present stable kinetic folding intermediates.

引用

页码：15105 / 15110

页数：6

共 52 条

[31] SEQUENCE-SPECIFIC H-1-NMR ASSIGNMENTS AND SECONDARY STRUCTURE OF THE STREPTOCOCCAL PROTEIN-G B2-DOMAIN
ORBAN, J
ALEXANDER, P
BRYAN, P
[J]. BIOCHEMISTRY, 1992, 31 (14) : 3604 - 3611
[32] STRUCTURE OF THE TRANSITION-STATE FOR THE FOLDING/UNFOLDING OF THE BARLEY CHYMOTRYPSIN INHIBITOR-2 AND ITS IMPLICATIONS FOR MECHANISMS OF PROTEIN-FOLDING
OTZEN, DE
ITZHAKI, LS
ELMASRY, NF
JACKSON, SE
FERSHT, AR
[J]. PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1994, 91 (22) : 10422 - 10425
[33] PACE CN, 1986, METHOD ENZYMOL, V131, P226
[34] Privalov P L, 1986, Methods Enzymol, V131, P4
[35] Privalov P L, 1979, Adv Protein Chem, V33, P167, DOI 10.1016/S0065-3233(08)60460-X
[36] PRIVALOV PL, 1988, ADV PROTEIN CHEM, V39, P191
[37] THERMODYNAMIC APPROACH TO PROBLEM OF STABILIZATION OF GLOBULAR PROTEIN STRUCTURE - CALORIMETRIC STUDY
PRIVALOV, PL
KHECHINA.NN
[J]. JOURNAL OF MOLECULAR BIOLOGY, 1974, 86 (03) : 665 - 684
[38] THE FOLDING OF HEN LYSOZYME INVOLVES PARTIALLY STRUCTURED INTERMEDIATES AND MULTIPLE PATHWAYS
RADFORD, SE
DOBSON, CM
EVANS, PA
[J]. NATURE, 1992, 358 (6384) : 302 - 307
[39] ANALYSIS OF THE THERMAL UNFOLDING OF PORCINE PROCARBOXYPEPTIDASE-A AND ITS FUNCTIONAL PIECES BY DIFFERENTIAL SCANNING CALORIMETRY
SANCHEZRUIZ, JM
LOPEZLACOMBA, JL
MATEO, PL
VILANOVA, M
SERRA, MA
AVILES, FX
[J]. EUROPEAN JOURNAL OF BIOCHEMISTRY, 1988, 176 (01): : 225 - 230
[40] UNIVERSAL NUCLEIC ACID-BINDING DOMAIN REVEALED BY CRYSTAL-STRUCTURE OF THE BACILLUS-SUBTILIS MAJOR COLD-SHOCK PROTEIN
SCHINDELIN, H
MARAHIEL, MA
HEINEMANN, U
[J]. NATURE, 1993, 364 (6433) : 164 - 168

← 1 2 3 4 5 6 →