PROTEIN FOLDING AND PROTEIN REFOLDING

被引：94

作者：

SECKLER, R ^{[1
]}

JAENICKE, R ^{[1
]}

机构：

[1] UNIV REGENSBURG, INST BIOPHYS & PHYS BIOCHEM, UNIV STR 31, W-8400 REGENSBURG, GERMANY

来源：

FASEB JOURNAL | 1992年 / 6卷 / 08期

关键词：

PROTEIN STRUCTURE; PROTEIN STABILITY; FOLDING; AGGREGATION; MOLECULAR CHAPERONES;

D O I：

10.1096/fasebj.6.8.1592207

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 functional three-dimensional structure of proteins is determined solely by their amino acid sequences. Protein folding occurs spontaneously beginning with the formation of local secondary structure concomitant with a compaction of the molecule. Secondary structure elements subsequently interact to form subdomains and domains stabilized by tertiary interactions. Disulfide bond formation, and cis-trans isomerization of X-Pro peptide bonds, as the rate-limiting folding reactions, are enzymatically catalyzed during protein folding in the cell. Although folding of domains is fast enough to occur cotranslationally in vivo, such vectorial folding on the ribosome is not essential for attainment of the native structure of a protein. Slow steps on the pathway to the functional protein structure are docking reactions of domains, association of subunits, or reshuffling reactions at the oligomer level. Aggregation as a competing side reaction is prevented, and the kinetic partition between competing polypeptide folding and translocation reactions is regulated by chaperone proteins binding to incompletely folded polypeptides.

引用

页码：2545 / 2552

页数：8

共 72 条

[1] PRINCIPLES THAT GOVERN FOLDING OF PROTEIN CHAINS [J].

ANFINSEN, CB .

SCIENCE, 1973, 181 (4096) :223-230

[2] PROTEIN DENATURATION AND THE PROPERTIES OF PROTEIN GROUPS [J].

ANSON, ML .

ADVANCES IN PROTEIN CHEMISTRY, 1945, 2 :361-386

[3] HOW DOES PROTEIN FOLDING GET STARTED [J].

BALDWIN, RL .

TRENDS IN BIOCHEMICAL SCIENCES, 1989, 14 (07) :291-294

[4] IDENTIFICATION OF A PROTEIN REQUIRED FOR DISULFIDE BOND FORMATION INVIVO [J].

BARDWELL, JCA ;

MCGOVERN, K ;

BECKWITH, J .

CELL, 1991, 67 (03) :581-589

[5] KINETIC CHARACTERIZATION OF EARLY IMMUNOREACTIVE INTERMEDIATES DURING THE REFOLDING OF GUANIDINE-UNFOLDED ESCHERICHIA-COLI TRYPTOPHAN SYNTHASE BETA-2 SUBUNITS [J].

BLONDELGUINDI, S ;

GOLDBERG, ME .

BIOCHEMISTRY, 1990, 29 (09) :2409-2417

[6] GROE FACILITATES REFOLDING OF CITRATE SYNTHASE BY SUPPRESSING AGGREGATION [J].

BUCHNER, J ;

SCHMIDT, M ;

FUCHS, M ;

JAENICKE, R ;

RUDOLPH, R ;

SCHMID, FX ;

KIEFHABER, T .

BIOCHEMISTRY, 1991, 30 (06) :1586-1591

[7] ALTERNATIVELY FOLDED STATES OF AN IMMUNOGLOBULIN [J].

BUCHNER, J ;

RENNER, M ;

LILIE, H ;

HINZ, HJ ;

JAENICKE, R ;

KIEFHABER, T ;

RUDOLPH, R .

BIOCHEMISTRY, 1991, 30 (28) :6922-6929

[8] DETECTION AND CHARACTERIZATION OF A FOLDING INTERMEDIATE IN BARNASE BY NMR [J].

BYCROFT, M ;

MATOUSCHEK, A ;

KELLIS, JT ;

SERRANO, L ;

FERSHT, AR .

NATURE, 1990, 346 (6283) :488-490

[9] ORIGINS OF STRUCTURE IN GLOBULAR-PROTEINS [J].

CHAN, HS ;

DILL, KA .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1990, 87 (16) :6388-6392

[10]

CREIGHTON TE, 1990, BIOCHEM J, V270, P1

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