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Arginine Decarboxylase from the pathogenic fungi, Colleotrichum gleosporosides : Purification and Properties

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dc.contributor.author Weerasooriya, M.K.B. en_US
dc.contributor.author Handagiripathira, H.M.N.L. en_US
dc.contributor.author Wijewickrama, G.T. en_US
dc.date.accessioned 2014-11-19T04:40:11Z
dc.date.available 2014-11-19T04:40:11Z
dc.date.issued 2003
dc.identifier.citation Weerasooriya, M.K.B., Handagiripathira, H.M.N.L. and Wijewickrama, G.T. 2003. Arginine Decarboxylase from the pathogenic fungi, Colleotrichum gleosporosides: Purification and Properties. Journal of Science of the University of Kelaniya, 01: 23-33.
dc.identifier.issn ISSN 1391-9210 en_US
dc.identifier.uri
dc.identifier.uri http://repository.kln.ac.lk/handle/123456789/3777
dc.description.abstract Arginine decarboxylase, a polyamine biosynthetic enzyme, was isolated from a phytopathogenic fungi, Colletotrichum gleosporoides, which causes Anthracnose in wide range of plants in many parts ofthe world. The enzyme was purified 25 fold with 16.7% recovery by elution through Sepharose 4B gel column and DEAE Cellulose ion exchange column. As determined by Sepharose 4B gel chromatography, the native molecular mass of the purified enzyme was ~265kDa. SDS-PAGE of the purified enzyme showed two bands around 65 kDa and ~25 kDa, suggesting that possibly this enzyme could be a hexamer of above two sub units. Optimum pH and temperature for the enzyme was 5.2 and 40�C respectively . Beyond 50�C enzyme activity slowly declined and was almost deactivated by 80�C. Approximate Km of the enzyme for the substrate arginine was 67mM. en_US
dc.publisher Journal of Science of the University of Kelaniya Sri Lanka en_US
dc.subject Anthracnose; Colletotrichum gleosporoides; Arginine decarboxylase; polyamine metabolism en_US
dc.title Arginine Decarboxylase from the pathogenic fungi, Colleotrichum gleosporosides : Purification and Properties
dc.type article en_US
dc.identifier.department Analytical Chemistry en_US


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