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Stability and reconstitution of pyruvate oxidase from lactobacillus plantarum: Dissection of the stabilizing effects of coenzyme binding and subunit interaction

✍ Scribed by Bernhard Risse; Günter Stempfer; Rainer Rudolph; Hans Möllering; Rainer Jaenicke

Book ID: 105356079
Publisher: Cold Spring Harbor Laboratory Press
Year: 1992
Tongue: English
Weight: 979 KB
Volume: 1
Category: Article
ISSN: 0961-8368
DOI: 10.1002/pro.5560011218

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✦ Synopsis

Abstract

Pyruvate oxidase from Lactobacillus plantarum is a homotetrameric flavoprotein with strong binding sites for FAD, TPP, and a divalent cation. Treatment with acid ammonium sulfate in the presence of 1.5 M KBr leads to the release of the cofactors, yielding the stable apoenzyme. In the present study, the effects of FAD, TPP, and Mn^2+^ on the structural properties of the apoenzyme and the reconstitution of the active holoenzyme from its constituents have been investigated.

As shown by circular dichroism and fluorescence emission, as well as by Nile red binding, the secondary and tertiary structures of the apoenzyme and the holoenzyme do not exhibit marked differences. The quaternary structure is stabilized significantly in the presence of the cofactors. Size‐exclusion high‐performance liquid chromatography and analytical ultracentrifugation demonstrate that the holoenzyme retains its tetrameric state down to 20 μg/mL, whereas the apoenzyme shows stepwise tetramer‐dimer‐monomer dissociation, with the monomer as the major component, at a protein concentration of <20 μg/mL.

In the presence of divalent cations, the coenzymes FAD and TPP bind to the apoenzyme, forming the inactive binary FAD or TPP complexes. Both FAD and TPP affect the quaternary structure by shifting the equilibrium of association toward the dimer or tetramer. High FAD concentrations exert significant stabilization against urea and heat denaturation, whereas excess TPP has no effect.

Reconstitution of the holoenzyme from its components yields full reactivation. The kinetic analysis reveals a compulsory sequential mechanism of cofactor binding and quaternary structure formation, with TPP binding as the first step. The binary TPP complex (in the presence of 1 mM Mn^2+^/TPP) is characterized by a dimer‐tetramer equilibrium transition with an association constant of K~a~ = 2 × 10^7^ M^−1^. The apoenzyme TPP complex dimer associates with the tetrameric holoenzyme in the presence of 10 μM FAD. This association step obeys second‐order kinetics with an association rate constant k = 7.4 × 10^3^ M^−1^ s^−1^ at 20 °C. FAD binding to the tetrameric binary TPP complex is too fast to be resolved by manual mixing.

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✍ Bernhard Risse; Günter Stempfer; Rainer Rudolph; Günter Schumacher; Rainer Jaeni 📂 Article 📅 1992 🏛 Cold Spring Harbor Laboratory Press 🌐 English ⚖ 798 KB

## Abstract Point mutations in the gene of pyruvate oxidase from __Lactobacillus plantarum__, with proline residue 178 changed to serine, serine 188 to asparagine, and alanine 458 to valine, as well as a combination of the three single point mutations, lead to a significant functional stabilization