Folding of aspartokinase-homoserine dehydrogenase I is dominated by tertiary interactions

Müller, K; Garel, Jean‐Renaud

doi:10.1021/bi00299a011

Cited by 11 publications

(8 citation statements)

References 23 publications

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“…A Faster Reaction Corresponding to the Major Folding Process Is Followed by a Slower Isomerization That Restores the Kinase Activity. In 3 M Gdn-HCl, AK-HDH exists as a stable (partially) folded monomeric species as seen from its fluorescence and circular dichroism properties (Garel et al, 1984;Müller & Garel, 1984a). The formation of this folded monomer from the unfolded chain has a half-life of 6.5 min in 3 M Gdn-HCl and of less than 0.5 min in 2 M Gdn-HCl (Müller & Garel, 1984a).…”

Section: Resultsmentioning

confidence: 99%

“…In 3 M Gdn-HCl, AK-HDH exists as a stable (partially) folded monomeric species as seen from its fluorescence and circular dichroism properties (Garel et al, 1984;Müller & Garel, 1984a). The formation of this folded monomer from the unfolded chain has a half-life of 6.5 min in 3 M Gdn-HCl and of less than 0.5 min in 2 M Gdn-HCl (Müller & Garel, 1984a). Upon dilution of AK-HDH from 6 M to less than 0.1 M Gdn-HCl, there is a fluorescence change too rapid to be measured after manual mixing; this holds even at lower temperature (down to 5 °C) or in the presence of glycerol [up to 30% (v/v)].…”

Section: Resultsmentioning

confidence: 99%

“…(i) Many large polypeptide chains appear as composed of several compact regions, which are supposed to correspond to independent folding segments (Wetlaufer, 1973;Schulz & Schirmer, 1979; Janin & Wodak, 1983); this is indeed the case with AK-HDH in which three compact regions exist (Fazel et al, 1983) and for which the presence of independently folding units has been shown (Dautry-Varsat & Garel, 1981; Müller & Garel, 1984a).…”

Section: The Slow Reactivationmentioning

confidence: 99%

“…e renaturation of an oligomeric protein from its unfolded and separated chains implies a mixture of folding and association reactions (Jaenicke, 1982(Jaenicke, , 1984Jaenicke & Rudolph, 1980). In the case of aspartokinase-homoserine dehydrogenase (AK-HDH),1 a tetrameric and bifunctional enzyme, the renaturation process could be decomposed into a succession of several steps (Garel & Dautry-Varsat, 1980a,b;Dautry-Varsat & Garel, 1981; Müller & Garel, 1984a): (i) a polypeptide chain acquires some organized structure, as seen from its fluorescence and circular dichroism, and forms a stable (partially) folded monomeric species; (ii) this (partially) folded species further isomerizes to yield an intermediate with full kinase activity and still a monomeric structure; (iii) two folded monomers then associate into a dimeric species that possesses a normal dehydrogenase activity; (iv) finally, two dimers as-tThis work was supported by the Centre National de la Recherche (UA 1129), the Instituí Pasteur, and the Université Paris 6 (UER 58).…”

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confidence: 99%

“…Both fragments can resume their functional structure after complete unfolding. The comparison between the kinetics of reactivation of the fragments and that of the entire chain shows that neither the mechanism nor the rate of renaturation is markedly affected by the removal of 30-40% at either end of the chain (Dautry-Varsat & Garel, 1981; Müller & Garel, 1984a). It seems then that, during the renaturation of AK-HDH, several segments along the polypeptide chain behave as independent folding units.…”

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confidence: 99%

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Mechanism of renaturation of a large protein, aspartokinase-homoserine dehydrogenase

Vaucheret¹,

Signon²,

Bras³

et al. 1987

Biochemistry

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The renaturation of aspartokinase-homoserine dehydrogenase and of some of its smaller fragments has been investigated after complete unfolding by 6 M guanidine hydrochloride. Fluorescence measurements show that a major folding reaction occurs rapidly (in less than a few seconds) after the protein has been transferred to native conditions and results in the shielding of the tryptophan residues from the aqueous solvent; this step also takes place in the fragments and probably corresponds to the independent folding of different segments along the polypeptide chain. The reappearance of the kinase activity, which is an index of the formation of "native" structure within a single chain, is much slower (a few minutes) and has the following properties: it is involved in a kinetic competition with the formation of aggregates; it has an activation energy of 22 +/- 5 kcal/mol; it is not related to a slow reaction in unfolding and thus probably not controlled by the cis-trans isomerization of X-Pro peptide bonds; its rate is inversely proportional to the solvent viscosity. It seems as if this reaction is limited by the mutual arrangement of the regions that have folded rapidly and independently. It is proposed that the mechanism where a fast folding of domains is followed by a slow pairing of folded domains could be generalized to other long chains composed of several domains; such a slow pairing of folded domains would correspond to a rate-limiting process specific to the renaturation of large proteins. The reappearance of the dehydrogenase activity measures the formation of a dimeric species. The dimerization can occur only after each chain has reached its "native" conformation.(ABSTRACT TRUNCATED AT 250 WORDS)

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Section: Resultsmentioning

confidence: 99%

Section: Resultsmentioning

confidence: 99%