Download PDF
Planta Med 1983; 48(8): 212-220
DOI: 10.1055/s-2007-969923
Research Articles

© Hippokrates Verlag Stuttgart

Partial Purification and Properties of (S)-Norlaudanosoline Synthase from Eschscholtzia tenuifolia Cell Cultures

H.-M. Schumacher1 , M. Rüffer1 , N. Nagakura2 , M. H. Zenk1
  • 1Lehrstuhl Pharmazeutische Biologie der Universität München, Federal Republic of Germany
  • 2Kobe Women's College of Pharmacy, Kobe, Japan
Further Information

Publication History

1983

Publication Date:
26 March 2007 (online)

  PDF Download  Permissions and Reprints

Abstract

A new enzyme, (S)-norlaudanosoline synthase, which catalyses the synthesis of (S)-norlaudanosoline from dopamine and 3,4-dihydroxyphenylacetaldehyde was isolated from the soluble protein extract of Eschscholtzia tenuifolia cell suspension cultures and purified approximately 40-fold. The apparent molecular weight of the enzyme is 15 500 Dalton. The pH optimum is 7.8, temperature optimum 40° C, apparent KM values for dopamine and dihydroxyphenyl-acetaldehyde are 1.5 mM and 0.7 mM respectively. The synthase shows high substrate specificity in that only the phenylacetaldehydes are transformed but not the phenylpyruvates. No apparent cofactor requirement could be demonstrated. By means of isoelectric focusing and disc-gel electrophoresis evidence was obtained for the existence of four norlaudanosoline synthase isoenzymes, none of which catalyses the reaction of dopamine with 3,4-dihydroxyphenylpyruvate. These enzymes are responsible for the synthesis of (S)-norlaudanosoline, the key intermediate in the formation of isoquinoline alkaloids occurring in the plant kingdom.

Key Word Index

Eschscholtzia tenuifolia - Papaveraceae - Cell Cultures - Alkaloid Biosynthesis - (S)-Norlaudanosoline Synthase

      >