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Please use this identifier to cite or link to this item: http://acervodigital.unesp.br/handle/11449/74149
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dc.contributor.authorGraminho, Eduardo Rezende-
dc.contributor.authorDa Silva, Ronivaldo Rodrigues-
dc.contributor.authorDe Freitas Cabral, Tatiana Pereira-
dc.contributor.authorArantes, Eliane Candiani-
dc.contributor.authorDa Rosa, Nathalia Gonsales-
dc.contributor.authorJuliano, Luiz-
dc.contributor.authorOkamoto, Debora Noma-
dc.contributor.authorDe Oliveira, Lilian Caroline Gonçalves-
dc.contributor.authorKondo, Marcia Yuri-
dc.contributor.authorJuliano, Maria Aparecida-
dc.contributor.authorCabral, Hamilton-
dc.date.accessioned2014-05-27T11:27:27Z-
dc.date.accessioned2016-10-25T18:40:51Z-
dc.date.available2014-05-27T11:27:27Z-
dc.date.available2016-10-25T18:40:51Z-
dc.date.issued2013-01-01-
dc.identifierhttp://dx.doi.org/10.1007/s12010-012-9974-3-
dc.identifier.citationApplied Biochemistry and Biotechnology, v. 169, n. 1, p. 201-214, 2013.-
dc.identifier.issn0273-2289-
dc.identifier.issn1559-0291-
dc.identifier.urihttp://hdl.handle.net/11449/74149-
dc.identifier.urihttp://acervodigital.unesp.br/handle/11449/74149-
dc.description.abstractThe purpose of this work was to purify a protease from Penicillium waksmanii and to determine its biochemical characteristics and specificity. The extracellular protease isolated that was produced by P. waksmanii is a serine protease that is essential for the reproduction and growth of the fungus. The protease isolated showed 32 kDa, and has optimal activity at pH 8.0 and 35 C towards the substrate Abz-KLRSSKQ-EDDnp. The protease is active in the presence of CaCl2, KCl, and BaCl, and partially inhibited by CuCl2, CoCl2 and totally inhibited by AlCl3 and LiCl. In the presence of 1 M urea, the protease remains 50 % active. The activity of the protease increases 60 % when it is exposed to 0.4 % nonionic surfactant-Triton X-100 and loses 10 % activity in the presence of 0.4 % Tween-80. Using fluorescence resonance energy transfer analysis, the protease showed the most specificity for the peptide Abz-KIRSSKQ-EDDnp with k cat/K m of 10,666 mM-1 s-1, followed by the peptide Abz-GLRSSKQ-EDDnp with a k cat/K m of 7,500 mM -1 s-1. Basic and acidic side chain-containing amino acids performed best at subsite S1. Subsites S2, S3, S′ 2, and S′ 1, S ′ 3 showed a preference for binding for amino acids with hydrophobic and basic amino acid side chain, respectively. High values of k cat/K m were observed for the subsites S2, S3, and S′ 2. The sequence of the N-terminus (ANVVQSNVPSWGLARLSSKKTGTTDYTYD) showed high similarity to the fungi Penicillium citrinum and Penicillium chrysogenum, with 89 % of identity at the amino acid level. © 2012 Springer Science+Business Media New York.en
dc.format.extent201-214-
dc.language.isoeng-
dc.sourceScopus-
dc.subjectFungal enzymes-
dc.subjectN-terminal Penicillium-
dc.subjectProtease-
dc.subjectPurification-
dc.subjectSpecificity-
dc.subjectBiochemical characteristics-
dc.subjectExtracellular protease-
dc.subjectFluorescence resonance energy transfer analysis-
dc.subjectN-terminals-
dc.subjectNonionic-
dc.subjectOptimal activity-
dc.subjectPenicillium chrysogenum-
dc.subjectPenicillium citrinum-
dc.subjectSerine protease-
dc.subjectSide-chains-
dc.subjectSubsites-
dc.subjectTween 80-
dc.subjectCalcium chloride-
dc.subjectCopper compounds-
dc.subjectEnergy transfer-
dc.subjectEnzyme activity-
dc.subjectNonionic surfactants-
dc.subjectPeptides-
dc.subjectUrea-
dc.subjectAmino acids-
dc.subjectaluminum chloride-
dc.subjectbarium chloride-
dc.subjectcalcium chloride-
dc.subjectcobalt chloride-
dc.subjectcopper chloride-
dc.subjectfungal enzyme-
dc.subjectpolysorbate 80-
dc.subjectpotassium chloride-
dc.subjectserine proteinase-
dc.subjecttriton x 100-
dc.subjecturea-
dc.subjectamino acid sequence-
dc.subjectamino terminal sequence-
dc.subjectbinding site-
dc.subjectcontrolled study-
dc.subjectenzyme activity-
dc.subjectenzyme analysis-
dc.subjectenzyme inhibition-
dc.subjectenzyme kinetics-
dc.subjectenzyme purification-
dc.subjectenzyme release-
dc.subjectenzyme specificity-
dc.subjectenzyme substrate-
dc.subjectenzyme synthesis-
dc.subjectfluorescence resonance energy transfer-
dc.subjectfungal reproduction-
dc.subjectfungus growth-
dc.subjectnonhuman-
dc.subjectPenicillium-
dc.subjectPenicillium waksmanii-
dc.subjectpH-
dc.subjectprotein cleavage-
dc.subjectprotein function-
dc.subjectspecies difference-
dc.subjectAmino Acid Sequence-
dc.subjectEnzyme Stability-
dc.subjectExtracellular Space-
dc.subjectFungal Proteins-
dc.subjectKinetics-
dc.subjectMolecular Sequence Data-
dc.subjectProtein Transport-
dc.subjectSerine Proteases-
dc.subjectSubstrate Specificity-
dc.subjectFungi-
dc.titlePurification, characterization, and specificity determination of a new serine protease secreted by penicillium waksmaniien
dc.typeoutro-
dc.contributor.institutionUniversidade de São Paulo (USP)-
dc.contributor.institutionUniversidade Estadual Paulista (UNESP)-
dc.contributor.institutionUniversidade Federal de São Paulo (UNIFESP)-
dc.description.affiliationDepartment of Pharmaceutical Sciences Faculty of Pharmaceutical Sciences of Ribeirão Preto University of São Paulo, Ribeirão Preto 14040-903-
dc.description.affiliationInstitute of Biosciences Letters and Exact Sciences Universidade Estadual Paulista, São José do Rio Preto 15054-000-
dc.description.affiliationDepartment of Biophysics Universidade Federal de São Paulo, São Paulo 04023-900-
dc.description.affiliationUnespInstitute of Biosciences Letters and Exact Sciences Universidade Estadual Paulista, São José do Rio Preto 15054-000-
dc.identifier.doi10.1007/s12010-012-9974-3-
dc.identifier.wosWOS:000314023100018-
dc.rights.accessRightsAcesso restrito-
dc.relation.ispartofApplied Biochemistry and Biotechnology-
dc.identifier.scopus2-s2.0-84873091920-
Appears in Collections:Artigos, TCCs, Teses e Dissertações da Unesp

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