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Research Article

Common amino acid domain among endopolygalacturonases of ascomycete fungi.

J P Keon, G Waksman
J P Keon
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G Waksman
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ABSTRACT

The endopolygalacturonase (EC 3.2.1.15) enzymes produced in vitro by three ascomycete fungi, Aspergillus niger, Sclerotinia sclerotiorum, and Colletotrichum lindemuthianum were studied by using thin-layer isoelectric focusing and activity stain overlay techniques. The polygalacturonases from A. niger and S. sclerotiorum consisted of numerous isoforms, whereas the endopolygalacturonase from C. lindemuthianum consisted of a single protein species. The most abundant endopolygalacturonase isoform produced by each of these organisms was purified and characterized. Biochemical parameters, including molecular weight, isoelectric point, kinetic parameters, temperature and pH optima, and thermal stability, were determined. Considerable differences in physical and chemical properties were demonstrated among these fungal polygalacturonases. Antibodies raised against individual proteins exhibited little cross-reaction, suggesting that these enzymes differ structurally as well as biochemically. In contrast, the analysis of the N-terminal amino acid sequences of the three proteins showed extensive homology, particularly in a region labeled domain 1 in which 84% of the amino acids were conserved.

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Common amino acid domain among endopolygalacturonases of ascomycete fungi.
J P Keon, G Waksman
Applied and Environmental Microbiology Aug 1990, 56 (8) 2522-2528; DOI:

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Common amino acid domain among endopolygalacturonases of ascomycete fungi.
J P Keon, G Waksman
Applied and Environmental Microbiology Aug 1990, 56 (8) 2522-2528; DOI:
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