Utilize este identificador para referenciar este registo: https://hdl.handle.net/1822/13560

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Campo DCValorIdioma
dc.contributor.authorSchnitzhofer, W-
dc.contributor.authorWeber, H.-J.-
dc.contributor.authorVršanská, M.-
dc.contributor.authorBiely, P.-
dc.contributor.authorPaulo, Artur Cavaco-
dc.contributor.authorGuebitz, G. M.-
dc.date.accessioned2011-09-13T14:59:17Z-
dc.date.available2011-09-13T14:59:17Z-
dc.date.issued2007-06-
dc.date.submitted2006-
dc.identifier.issn0141-0229por
dc.identifier.urihttps://hdl.handle.net/1822/13560-
dc.description.abstractSclerotium rolfsii (strain CBS 350.80) was found to produce extraordinary high amounts of polygalacturonases (PGs). Two of these extracellular enzymes were purified by a recently introduced preparative electrophoretic device (isoelectric focusing mode of free flow electrophoresis). PG 1 (39.5 kDa, pI 6.5) and PG 2 (38 kDa, pI 5.4) exhibited quite similar properties, they were found to be both endo-acting enzymes. Both PGs cleaved penta- and trigalacturonic acid while tetragalacturonic acid was only cleaved when trigalacturonic acid was present. The latter substrate was hydrolysed much faster by PG 2. Both enzymes were active on pectins with different degrees of esterification, they were sensitive towards Ca-cations and not glycosylated. The kinetic properties were measured by viscosimetry with polygalacturonic acid as a substrate. NMR experiments on a model substrate revealed an inverting mechanism of carbohydrate hydrolysis for both enzymes.por
dc.language.isoengpor
dc.publisherElsevier 1por
dc.rightsopenAccesspor
dc.subjectPolygalacturonasepor
dc.subjectFFEpor
dc.subjectPurificationpor
dc.subjectPectinasepor
dc.subjectPlant pathogen funguspor
dc.titlePurification and mechanistic characterisation of two polygalacturonases from Sclerotium rolfsiipor
dc.typearticlepor
dc.peerreviewedyespor
dc.relation.publisherversionhttp://www.sciencedirect.com/science/article/pii/S0141022906005473por
sdum.publicationstatuspublishedpor
oaire.citationStartPage1739por
oaire.citationEndPage1747por
oaire.citationIssue7por
oaire.citationTitleEnzyme and Microbial Technologypor
oaire.citationVolume40por
dc.identifier.doi10.1016/j.enzmictec.2006.11.005por
dc.subject.wosScience & Technologypor
sdum.journalEnzyme and Microbial Technologypor
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