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Synergy of Ion Exchange and Covalent Reaction: Immobilization of Penicillin G Acylase on Heterofunctional Amino-Vinyl Sulfone Agarose

dc.contributor.authorda Rocha, Thays N.
dc.contributor.authorMorellon-Sterling, Roberto
dc.contributor.authorGonçalves, Luciana R. B.
dc.contributor.authorBolívar Bolívar, Juan Manuel
dc.contributor.authorAlcántara León, Andrés Rafael
dc.contributor.authorRocha Martín, Javier
dc.contributor.authorFernández-Lafuente, Roberto
dc.date.accessioned2024-07-05T15:24:07Z
dc.date.available2024-07-05T15:24:07Z
dc.date.issued2023-01-09
dc.description.abstractAgarose-vinyl sulfone (VS) beads have proven to be a good support to immobilize several enzymes. However, some enzymes are hardly immobilized on it. This is the case of penicillin G acylase (PGA) from Escherichia coli, which is immobilized very slowly on this support (less than 10% in 24 h). This enzyme is also not significantly adsorbed in aminated MANAE-agarose beads, an anionic exchanger. In this study, MANAE-agarose beads were modified with divinyl sulfone (DVS) to produce MANAE-vinyl sulfone (VS) agarose beads. When PGA was immobilized on this support, the enzyme was fully immobilized in less than 1.5 h. PGA cannot be released from the support by incubation at high ionic strength, suggesting that the enzyme was rapidly immobilized in a covalent fashion. Considering that the amount of reactive VS groups was only marginally increased, the results indicated some cooperative effect between the anion exchange on the amine groups of the support, probably as the first step of the process, and the covalent attachment of the previously adsorbed PGA molecules. The covalent reaction of the previously adsorbed enzyme molecules proceeds much more efficiently than that of the free enzyme, due to the proximity of the reactive groups of the support and the enzyme. Finally, the steps of immobilization, incubation, and blocking with different agents were studied to determine the effects on final activity/stability. The stability of PGA immobilized on this new catalyst was improved with respect to the VS-agarose prepared at low ionic strength.
dc.description.departmentDepto. de Ingeniería Química y de Materiales
dc.description.departmentDepto. de Química en Ciencias Farmacéuticas
dc.description.departmentDepto. de Bioquímica y Biología Molecular
dc.description.facultyFac. de Ciencias Químicas
dc.description.facultyFac. de Farmacia
dc.description.facultyFac. de Ciencias Biológicas
dc.description.fundingtypeDescuento UCM
dc.description.refereedTRUE
dc.description.statuspub
dc.identifier.citationda Rocha, T.N.; Morellon-Sterling, R.; Gonçalves, L.R.B.; Bolivar, J.M.; Alcántara, A.R.; Rocha-Martin, J.; Fernández-Lafuente, R. Synergy of Ion Exchange and Covalent Reaction: Immobilization of Penicillin G Acylase on Heterofunctional Amino-Vinyl Sulfone Agarose. Catalysts 2023, 13, 151. https://doi.org/10.3390/catal13010151
dc.identifier.doi10.3390/catal13010151
dc.identifier.issn2073-4344
dc.identifier.officialurlhttps://doi.org/10.3390/catal13010151
dc.identifier.relatedurlhttps://www.mdpi.com/2073-4344/13/1/151
dc.identifier.urihttps://hdl.handle.net/20.500.14352/105719
dc.issue.number1
dc.journal.titleCatalysts
dc.language.isoeng
dc.page.final151
dc.page.initial151
dc.publisherMDPI
dc.rightsAttribution 4.0 Internationalen
dc.rights.accessRightsopen access
dc.rights.urihttp://creativecommons.org/licenses/by/4.0/
dc.subject.cdu577.1
dc.subject.keywordIon exchanger
dc.subject.keywordVinyl sulfone-activated support
dc.subject.keywordHeterofunctional supports
dc.subject.keywordSynergy in enzyme immobilization
dc.subject.keywordCovalent enzyme immobilization
dc.subject.keywordPenicillin G acylase
dc.subject.ucmCiencias
dc.subject.ucmBioquímica (Química)
dc.subject.unesco2302 Bioquímica
dc.titleSynergy of Ion Exchange and Covalent Reaction: Immobilization of Penicillin G Acylase on Heterofunctional Amino-Vinyl Sulfone Agarose
dc.typejournal article
dc.type.hasVersionVoR
dc.volume.number13
dspace.entity.typePublication
relation.isAuthorOfPublicationdd41e7a5-3013-4b28-8263-915921ecf30a
relation.isAuthorOfPublicationc0d1193e-3161-4c69-af69-830b32f61932
relation.isAuthorOfPublication9d7ac6de-a596-4647-a7fa-3a1c143055e4
relation.isAuthorOfPublication.latestForDiscoverydd41e7a5-3013-4b28-8263-915921ecf30a

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