Identification and characterization of glycolate oxidase and related enzymes from the endocyanotic alga Cyanophora paradoxa and from pea leaves

Identification and characterization of glycolate oxidase and related enzymes from the endocyanotic alga Cyanophora paradoxa and from pea leaves

Glycolate oxidase (GO) has been identified in the endocyanom Cyanophora paradoxa which has peroxisome-like organelles and cyanelles instead of chloroplasts. The enzyme used or formed equimolar amounts of O2 or H2O2 and glyoxylate, respectively. Aerobically, the enzyme did not reduce the artificial e...

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Veröffentlicht in:Plant physiology (Bethesda) 1992-03, Vol.98 (3), p.887-893
Hauptverfasser: Betsche, T. (Centre de Cadarache, Saint Paul lez Durance, France), Schaller, D, Melkonian, M
Format: Artikel
Sprache:eng
Schlagworte:
ACTIVIDAD ENZIMATICA
ACTIVITE ENZYMATIQUE
Algae
Biological and medical sciences
CHLOROPLASTE
CLOROPLASTO
Cyanophora
CYANOPHYTA
Dehydrogenases
Enzymes
FEUILLE
Fundamental and applied biological sciences. Psychology
Glycolates
Glyoxylates
HOJAS
Kinetics
Life Sciences & Biomedicine
Metabolism
OXIDACION
Oxidases
OXIDORREDUCTASAS
OXYDATION
OXYDOREDUCTASE
Peas
PISUM SATIVUM
Plant physiology and development
Plant Sciences
Plants
PURIFICACION
PURIFICATION
Science & Technology
VIA METABOLICA FOTORESPIRACION
VOIE METABOLISME PHOTORESPIRATOIRE
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Zusammenfassung:Glycolate oxidase (GO) has been identified in the endocyanom Cyanophora paradoxa which has peroxisome-like organelles and cyanelles instead of chloroplasts. The enzyme used or formed equimolar amounts of O2 or H2O2 and glyoxylate, respectively. Aerobically, the enzyme did not reduce the artificial electron acceptor dichlorophenol indophenol. However, after an inhibitor of glycolate dehydrogenase, KCN (2 millimolar), was added to the assay medium, considerable aerobic glycolate:dichlorophenol indophenol reductase activity was detectable. The leaf GO inhibitor 2-hydroxybutynoate (30 micromolar), which binds irreversibly to the flavin moiety of the active site of leaf GO, inhibited Cyanophora GO and pea (Pisum sativum L) GO to the same extent. This suggests that the active sites of both enzymes are similar. Cyanophora GO and pea GO cannot oxidize D-lactate. In contrast to GO from pea or other organisms, the affinity of Cyanophora GO for L-lactate is very low (Km 25 millimolar). Another important difference is that Cyanophora GO produced sigmoidal kinetics with O2 as varied substrate, whereas pea GO produced normal Michaelis-Menten kinetics. It is concluded that there is considerable inhomogeneity among the glycolate-oxidizing enzymes from Cyanophora, pea, and other organisms. The specific catalase activity in Cyanophora was only one-tenth of that in leaves. NADH- and NADPH-dependent hydroxypyruvate reductase (HPR) and glyoxylate reductase activities were detected in Cyanophora. NADH-HPR was markedly inhibited by hydroxypyruvate above 0.5 millimolar. Variable substrate inhibition was observed with glyoxylate in homogenates from different algal cultures. R is proposed that Cyanophora has multiple forms of HPR and glyoxylate reductase, but no enzyme clearly resembling leaf peroxisomal HPR was identified in these homogenates. Moreover, no serine:glyoxylate aminotransferase activity was detected. These results collectively indicate the possibility that the glycolate metabolism in Cyanophora deviates from that in leaves
ISSN:0032-0889
1532-2548
DOI:10.1104/pp.98.3.887