Isolation and characterization of wheat peroxidase isoenzyme B1 |
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Authors: | Zdeněk Zmrhal Ivana Macháčková |
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Affiliation: | Institute of Plant Nutrition, Institute of Crop Production, Prague 6, Czechoslovakia |
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Abstract: | Two pure peroxidase isoenzymes B1 and D4 were isolated from the upper parts of 10-day-old wheat seedlings by means of gel and ion-exchange chromatography. Their MWs were 85000 and 24000 respectively. B1 was unstable and under various conditions it was converted to another isoenzyme, electrophoretically identical with D4. B1 contains about 40% of neutral sugars: 17.2% arabinose, 15.3% galactose, 5% glucose and traces of mannose. D4 is free of neutral sugars. None of the isoenzymes contained amino sugars. B1 oxidizes ferulic and p-coumaric acids. This oxidation has two pH optima of 4.4 and 5.4–5.6 and is inhibited by high concentrations of substrates, cyanide and azide. B1 oxidizes IAA in the presence of phenolic cofactor and Mn2+ ions. IAA oxidation has two pH optima of 4.5 and 5.6 and is inhibited by high substrate concentration, cyanide and azide, and by a number of indole derivatives. The main products of IAA oxidation are 3-methyleneoxindole and indole-3-methanol. o- and p- diphenols induce a lag period prior to IAA oxidation. Ferulic acid is oxidized during this lag period, probably to a dimer. B1 is able to produce H2O2 from oxygen. Mn2+ ions, a phenolic cofactor and an electron donor (IAA or NADH) are needed. B1 oxidizes α-keto-γ- methylmercaptobutyric acid to ethylene. D4 has a low peroxidatic activity and is inactive as an IAA oxidase. Thus B1 is probably an active cell wall-bound peroxidase isoenzyme, whereas D4 is its decomposition product. |
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Keywords: | IAA: indole-3-acetic acid KMBA: α-keto-γ-methylmercaptobutyric acid FA : ferulic(3-methoxy-4-hydroxy-cinnamic)acid MOI: 3-methyleneoxindole NADH: reduced nicotinamide adenine nucleotide SDS: sodium dodecyl sulphate HRP: horseradish peroxidase. Gramineae peroxidase isoenzymes indole-3-acetic acid phenolic substances ethylene. |
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