Purification and characteristics of an enzyme with both bilirubin oxidase and laccase activities from mycelium of the basidiomycete Pleurotus ostreatus

A homogenous enzyme with both bilirubin oxidase and laccase activities was isolated from a submerged culture of the basidiomycete Pleurotus ostreatus mycelium and characterized. The yield of the enzyme was 127 μg/g dry biomass of the mycelium. The specific activity of the enzyme was 21 and 261 U/mg...

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Published inBiochemistry (Moscow) Vol. 74; no. 9; pp. 1027 - 1034
Main Authors Pakhadnia, Y. G., Malinouski, N. I., Lapko, A. G.
Format Journal Article
LanguageEnglish
Published Dordrecht SP MAIK Nauka/Interperiodica 01.09.2009
Springer Nature B.V
Subjects
Amino acids
Biochemistry
Biomedical and Life Sciences
Biomedicine
Bioorganic Chemistry
Catalysis
Enzyme Stability
Enzymes
Fungi
Hydrogen-Ion Concentration
Kinetics
Laccase - isolation & purification
Laccase - metabolism
Life Sciences
Microbiology
Oxidoreductases Acting on CH-CH Group Donors - isolation & purification
Oxidoreductases Acting on CH-CH Group Donors - metabolism
Phenols
Pleurotus - enzymology
Pleurotus - growth & development
Spectrometry, Mass, Electrospray Ionization
Substrate Specificity
Substrates
Tandem Mass Spectrometry
mycelium
bilirubin oxidase
oxidoreductase
laccase
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Summary:A homogenous enzyme with both bilirubin oxidase and laccase activities was isolated from a submerged culture of the basidiomycete Pleurotus ostreatus mycelium and characterized. The yield of the enzyme was 127 μg/g dry biomass of the mycelium. The specific activity of the enzyme was 21 and 261 U/mg to bilirubin and to a laccase substrate ABTS, respectively. The intracellular phenol oxidase from the P. ostreatus mycelium was identified as bilirubin oxidase with the amino acid sequence highly homologous to that of the pox2 gene-encoded product. The enzyme displayed the maximal laccase activity at 50–55°C to all substrates examined, whereas the pH optimum was substrate-dependent and changed from 3.0 for ABTS to 7.0 for syringaldazine and guaiacol. The enzyme maintained catalytic activity within a broad pH range but was inactivated at pH 4.0. The enzyme was thermostable but very sensitive to metal chelating inhibitors. Trypan Blue (5 mg/liter) was completely decolorizated upon 3 h of incubation with the bilirubin oxidase (20 mU/ml) at room temperature.
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ISSN:0006-2979
1608-3040
DOI:10.1134/S0006297909090119