Cloning, expression, purification and characterization of recombinant (+)-germacrene D synthase from Zingiber officinale |
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Authors: | Picaud Sarah Olsson Mikael E Brodelius Maria Brodelius Peter E |
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Institution: | Department of Chemistry and Biomedical Sciences, University of Kalmar, SE-39182 Kalmar, Sweden. |
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Abstract: | A cDNA clone encoding a sesquiterpene synthase, (+)-germacrene D synthase, has been isolated from ginger (Zingiber officinale). The full-length cDNA (AY860846) contains a 1650-bp open reading frame coding for 550 amino acids (63.8kDa) with a theoretical pI=5.59. The deduced amino acid sequence is 30-46% identical with sequences of other sesquiterpene synthases from angiosperms. The recombinant enzyme, produced in Escherichia coli, catalyzed the formation of a major product, (+)-germacrene D (50.2% of total sesquiterpenoids produced) and a co-product, germacrene B (17.1%) and a number of minor by-products. The optimal pH for the recombinant enzyme is around 7.5. Substantial (+)-germacrene D synthase activity is observed in the presence of Mg2+, Mn2+, Ni2+ or Co2+, while the enzyme is inactive when Cu2+ or Zn2+ is used. The Km- and kcat-values are 0.88 microM and 3.34 x 10(-3) s(-1), respectively. A reaction mechanism involving a double 1,2-hydride shift has been established using deuterium labeled substrates in combination with GC-MS analysis. |
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Keywords: | cDNA cloning Enzyme characterization (+)-Germacrene D synthase Recombinant protein Sesquiterpenes Zingiber officinale |
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