Title of article
Determination of phenolic compounds using recombinant tyrosinase from Streptomyces antibioticus Original Research Article
Author/Authors
Katrin Streffer، نويسنده , , Erik Vijgenboom، نويسنده , , Armand W.J.W Tepper، نويسنده , , Alexander Makower، نويسنده , , Frieder W Scheller، نويسنده , , Gerard W Canters، نويسنده , , Ulla Wollenberger، نويسنده ,
Issue Information
روزنامه با شماره پیاپی سال 2001
Pages
10
From page
201
To page
210
Abstract
Properties of Streptomyces antibioticus tyrosinase and the implementation of the enzyme in a biosensor for the detection of phenolic compounds were investigated. The tyrosinase from S. antibioticus is a monomer and has a molecular weight of 30.6 kD. The specific activity is about 5 U/mg with catechol as substrate and 1225 U/mg with l-dopa as substrate. The activity of tyrosinase upon long-term storage is best maintained in buffer at temperatures of −80 or +4°C. Storage at −18°C, with or without glycerol, resulted in quick enzyme inactivation.
For the construction of the sensor bi-enzymatic substrate recycling was exploited. Quinoprotein glucose dehydrogenase (GDH) and tyrosinase were immobilised in polyvinyl alcohol and coupled to a Clark-type oxygen electrode that allowed for monitoring of the oxygen consumption during catechol conversion. This design of the sensor facilitates the determination of phenolic compounds in the nanomolar range. The lower limit of detection for l-dopa, dopamine, and adrenalin was 5 nM.
Keywords
Phenolic compounds , Glucose dehydrogenase , Biosensor , Tyrosinase , Substituted catechols
Journal title
Analytica Chimica Acta
Serial Year
2001
Journal title
Analytica Chimica Acta
Record number
1032146
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