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      Plate assay for determining the time of production of protease, cellulase, and pectinases by germinating fungal spores.

      Analytical Biochemistry
      Cellulase, biosynthesis, Glycoside Hydrolases, Kinetics, Mitosporic Fungi, enzymology, physiology, Peptide Hydrolases, Polygalacturonase, Spores, Fungal

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          Abstract

          A new method for detecting enzymes produced by fungal spores during germination is described here. With this method, the production of enzymes such as protease, cellulase, or pectinase can be correlated with the extent of spore germination. Germination is studied in vitro on agar-based media containing protein, cellulose, or pectin. The spores are immobilized on a permeable membrane mounted on the substrate-containing medium. At various times after inoculation the membrane-bound spores are removed and the medium is stained. The extent of germination is assessed by microscopic examination of the spores and the presence of active hydrolytic enzymes is revealed by the staining. The staining methods are sensitive; detection limits are 1 X 10(-3) unit of cellulase; 2 X 10(-4) unit of protease; 3 X 10(-3) unit of pectin lyase; 3.5 units of polygalacturonase; 2 X 10(-3) unit of pectin methyl esterase. The method has been demonstrated by studying the production of enzymes by germinating conidia of Botrytis cinerea. Cellulase and protease were present before any spores germinated. Pectin lyase was first observed when at least 80% of the spores had germinated. Pectin methyl esterase and polygalacturonase were not produced by the spores.

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          Author and article information

          Journal
          3913330
          10.1016/0003-2697(85)90184-8

          Chemistry
          Cellulase,biosynthesis,Glycoside Hydrolases,Kinetics,Mitosporic Fungi,enzymology,physiology,Peptide Hydrolases,Polygalacturonase,Spores, Fungal

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