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dc.contributor.authorAlmeida, Maíra N.de
dc.contributor.authorFalkoski, Daniel L.
dc.contributor.authorGuimarães, Valéria M.
dc.contributor.authorRamos, Humberto Josué de O.
dc.contributor.authorVisser, Evan M.
dc.contributor.authorMaitan-Alfenas, Gabriela P.
dc.contributor.authorRezende, Sebastião T. de
dc.date.accessioned2018-03-08T14:53:40Z
dc.date.available2018-03-08T14:53:40Z
dc.date.issued2013-06-08
dc.identifier.issn09608524
dc.identifier.urihttps://doi.org/10.1016/j.biortech.2013.06.021
dc.identifier.urihttp://www.locus.ufv.br/handle/123456789/18128
dc.description.abstractA novel multienzyme complex, E1 C , and a free endoglucanase, E2 (GH5), from Fusarium verticillioides were purified. The E1 C contained two endoglucanases (GH6 and GH10), one cellobiohydrolase (GH7) and one xylanase (GH10). Maximum activity was observed at 80 °C for both enzymes and they were thermostable at 50 and 60 °C. The activation energies for E1 C and E2 were 21.3 and 27.5 kJ/mol, respectively. The K M for E1 C was 10.25 g/L while for E2 was 6.58 g/L. Both E1 C and E2 were activated by Mn 2+ and CoCl 2 while they were inhibited by SDS, CuSO 4 , FeCl 3 , AgNO 4 , ZnSO 4 and HgCl 2 . E1 C and E2 presented endo-b-1,3–1,4-glucanase activity. E1 C presented crescent activity towards cellopentaose, cellotetraose and cellotriose. E2 hydrolyzed the substrates cellopentaose, cellotetraose and cellotriose with the same efficiency. E1 C showed a higher stability and a better hydrolysis performance than E2, suggesting advantages resulting from the physical interaction between proteins.en
dc.formatpdfpt-BR
dc.language.isoengpt-BR
dc.publisherBioresource Technologypt-BR
dc.relation.ispartofseriesv. 143, p. 413-422, September 2013pt-BR
dc.rightsPublished by Elsevier Ltd.pt-BR
dc.subjectMultienzyme complexpt-BR
dc.subjectEndoglucanasept-BR
dc.subjectCellobiohydrolasept-BR
dc.subjectXylanasept-BR
dc.subjectFusarium verticillioidespt-BR
dc.titleCharacteristics of free endoglucanase and glycosidases multienzyme complex from Fusarium verticillioidesen
dc.typeArtigopt-BR
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