Cofactor A is a molecular chaperone required for beta-tubulin folding: Functional and structural characterization

被引：53

作者：

Melki, R ^{[1
]}

Rommelaere, H ^{[1
]}

Leguy, R ^{[1
]}

Vandekerckhove, J ^{[1
]}

Ampe, C ^{[1
]}

机构：

[1] STATE UNIV GHENT VIB, FAC MED, DEPT BIOCHEM, B-9000 GHENT, BELGIUM

来源：

BIOCHEMISTRY | 1996年 / 35卷 / 32期

关键词：

D O I：

10.1021/bi960788r

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：

Actin and tubulin polypeptide drains acquire their native conformation in the presence of the chaperonin containing TCP-1 (CCT) and, in the case of alpha- and beta-tubulin additional protein cofactors. We recently identified one of these cofactors, termed cofactor A, that is required for the proper folding of the beta-tubulin chain [Gao et al. (1994) J. Cell. Biol. 125, 989-996]. We show here that cofactor A, a monomeric protein that has no measurable affinity for nucleotides, is a highly conserved protein among vertebrates. Its NH2-terminal region is essential for the structural integrity of the protein and consequently for its activity. We demonstrate that cofactor A does not interact with CCT nor does it affect the intrinsic ATPase activity of CCT, alone or in the presence of different target proteins. Thus, unlike GroES, cofactor A does not modulate or coordinate ATP hydrolysis. It does not act as a nucleotide exchange factor or a catalyst in tubulin folding. Rather, we demonstrate that cofactor A participates in the tubulin folding process by interacting with a folding intermediate of beta-tubulin that is released from CCT. Our data imply that cofactor A is a chaperone involved in tubulin folding.

引用

页码：10422 / 10435

页数：14

共 54 条

[1] RBL2P, A YEAST PROTEIN THAT BINDS TO BETA-TUBULIN AND PARTICIPATES IN MICROTUBULE FUNCTION IN-VIVO [J].

ARCHER, JE ;

VEGA, LR ;

SOLOMON, F .

CELL, 1995, 82 (03) :425-434

[2] CHARACTERIZATION OF A FUNCTIONAL GROEL(14)(GROES(7))(2) CHAPERONIN HETERO-OLIGOMER [J].

AZEM, A ;

KESSEL, M ;

GOLOUBINOFF, P .

SCIENCE, 1994, 265 (5172) :653-656

[3] BINDING OF A CHAPERONIN TO THE FOLDING INTERMEDIATES OF LACTATE-DEHYDROGENASE [J].

BADCOE, IG ;

SMITH, CJ ;

WOOD, S ;

HALSALL, DJ ;

HOLBROOK, JJ ;

LUND, P ;

CLARKE, AR .

BIOCHEMISTRY, 1991, 30 (38) :9195-9200

[4] TRANSIENT ASSOCIATION OF NEWLY SYNTHESIZED UNFOLDED PROTEINS WITH THE HEAT-SHOCK GROEL PROTEIN [J].

BOCHKAREVA, ES ;

LISSIN, NM ;

GIRSHOVICH, AS .

NATURE, 1988, 336 (6196) :254-257

[5]

BOCHKAREVA ES, 1992, J BIOL CHEM, V267, P6796

[6] THE CRYSTAL-STRUCTURE OF THE BACTERIAL CHAPERONIN GROEL AT 2.8-ANGSTROM [J].

BRAIG, K ;

OTWINOWSKI, Z ;

HEGDE, R ;

BOISVERT, DC ;

JOACHIMIAK, A ;

HORWICH, AL ;

SIGLER, PB .

NATURE, 1994, 371 (6498) :578-586

[7] A POLYPEPTIDE BOUND BY THE CHAPERONIN GROEL IS LOCALIZED WITHIN A CENTRAL CAVITY [J].

BRAIG, K ;

SIMON, M ;

FURUYA, F ;

HAINFELD, JF ;

HORWICH, AL .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1993, 90 (09) :3978-3982

[8] CARBOXY-TERMINAL REGIONS ON THE SURFACE OF TUBULIN AND MICROTUBULES - EPITOPE LOCATIONS OF YOL1/34, DM1A AND DM1B [J].

BREITLING, F ;

LITTLE, M .

JOURNAL OF MOLECULAR BIOLOGY, 1986, 189 (02) :367-370

[9]

CHANDRASEKHAR GN, 1986, J BIOL CHEM, V261, P2414

[10] LOCATION OF A FOLDING PROTEIN AND SHAPE CHANGES IN GROEL-GROES COMPLEXES IMAGED BY CRYOELECTRON MICROSCOPY [J].

CHEN, S ;

ROSEMAN, AM ;

HUNTER, AS ;

WOOD, SP ;

BURSTON, SG ;

RANSON, NA ;

CLARKE, AR ;

SAIBIL, HR .

NATURE, 1994, 371 (6494) :261-264

← 1 2 3 4 5 6 →