COLLAPSED INTERMEDIATES IN THE RECONSTITUTION OF DIMERIC ASPARTATE-AMINOTRANSFERASE FROM ESCHERICHIA-COLI

被引：23

作者：

LEISTLER, B ^{[1
]}

HEROLD, M ^{[1
]}

KIRSCHNER, K ^{[1
]}

机构：

[1] UNIV BASEL, BIOCTR, DEPT BIOPHYS CHEM, KLINGELBERGSTR 70, CH-4056 BASEL, SWITZERLAND

来源：

EUROPEAN JOURNAL OF BIOCHEMISTRY | 1992年 / 205卷 / 02期

关键词：

D O I：

10.1111/j.1432-1033.1992.tb16818.x

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：

Aspartate aminotransferase from Escherichia coli, which had been denatured by guanidinium chloride, refolded and reassembled to active dimers in two distinct phases. The unfolded monomer U collapsed within 20 s to an intermediate I* that was inactive, fluoresced more strongly than, but had the same peptide CD signal as the native dimer. The formation of crosslinkable dimers, as well as the recovery of enzyme activity, occurred with a biphasic progress curve which was independent of protein concentration. The half-lives of the two phases were 100 s and 2000 s. The data are consistent with a three-step mechanism, in which the overall rate of reassembly is determined by an isomerization of I* to the assembly-competent monomer M. The latter does not accumulate because it dimerizes rapidly to the active enzyme (D). Reassembly of the enzyme from the compact intermediate M*, which is stable at 1.0 M guanidinium chloride, also proceeded in a rapid and a slow phase. Moreover, the formation of M* from the unfolded state was rapid, whereas its refolding to the native dimer was slow. Both the transient intermediate I* and the equilibrium inter-mediate M* qualify as 'collapsed intermediate' or 'molten globule' states.

引用

页码：603 / 611

页数：9

共 34 条

[1]

[Anonymous], 1989, PROTEIN STRUCTURE PR

[2] KINETICS AND IMPORTANCE OF THE DIMERIZATION STEP IN THE FOLDING PATHWAY OF THE BETA-2 SUBUNIT OF ESCHERICHIA-COLI TRYPTOPHAN SYNTHASE [J].

BLOND, S ;

GOLDBERG, ME .

JOURNAL OF MOLECULAR BIOLOGY, 1985, 182 (04) :597-606

[3] CONSIDERATION OF POSSIBILITY THAT SLOW STEP IN PROTEIN DENATURATION REACTIONS IS DUE TO CIS-TRANS ISOMERISM OF PROLINE RESIDUES [J].

BRANDTS, JF ;

HALVORSON, HR ;

BRENNAN, M .

BIOCHEMISTRY, 1975, 14 (22) :4953-4963

[4]

CHRISTENSEN H, 1991, EUR BIOPHYS J, V19, P221, DOI 10.1007/BF00183530

[5]

EBERHARD M, 1990, COMPUT APPL BIOSCI, V6, P213

[6] THE MECHANISM OF PROTEIN FOLDING - IMPLICATIONS OF INVITRO REFOLDING MODELS FOR DENOVO PROTEIN FOLDING AND TRANSLOCATION IN THE CELL [J].

FISCHER, G ;

SCHMID, FX .

BIOCHEMISTRY, 1990, 29 (09) :2205-2212

[7] THE CLONING AND SEQUENCE-ANALYSIS OF THE ASPC AND TYRB GENES FROM ESCHERICHIA-COLI-K12 - COMPARISON OF THE PRIMARY STRUCTURES OF THE ASPARTATE-AMINOTRANSFERASE AND AROMATIC AMINOTRANSFERASE OF ESCHERICHIA-COLI WITH THOSE OF THE PIG ASPARTATE-AMINOTRANSFERASE ISOENZYMESN [J].

FOTHERINGHAM, IG ;

DACEY, SA ;

TAYLOR, PP ;

SMITH, TJ ;

HUNTER, MG ;

FINLAY, ME ;

PRIMROSE, SB ;

PARKER, DM ;

EDWARDS, RM .

BIOCHEMICAL JOURNAL, 1986, 234 (03) :593-604

[8] REFOLDING OF ESCHERICHIA-COLI DIHYDROFOLATE-REDUCTASE - SEQUENTIAL FORMATION OF SUBSTRATE BINDING-SITES [J].

FRIEDEN, C .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1990, 87 (12) :4413-4416

[9] REFOLDING AND REACTIVATION OF LIVER ALCOHOL-DEHYDROGENASE AFTER DISSOCIATION AND DENATURATION IN 6M GUANIDINE-HYDROCHLORIDE [J].

GERSCHITZ, J ;

RUDOLPH, R ;

JAENICKE, R .

EUROPEAN JOURNAL OF BIOCHEMISTRY, 1978, 87 (03) :591-599

[10] ANALYSIS OF THE RECONSTITUTION OF OLIGOMERIC ENZYMES BY CROSS-LINKING WITH GLUTARALDEHYDE - KINETICS OF REASSOCIATION OF LACTIC-DEHYDROGENASE [J].

HERMANN, R ;

JAENICKE, R ;

RUDOLPH, R .

BIOCHEMISTRY, 1981, 20 (18) :5195-5201

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