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Use este identificador para citar ou linkar para este item: https://repositorio.inpa.gov.br/handle/1/39547
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dc.contributor.authorPessoa, Vitor Alves-
dc.contributor.authorSoares, L.B.N-
dc.contributor.authorSilva, Gerlane L.-
dc.contributor.authorVasconcelos, Alice S.-
dc.contributor.authorSilva, JF-
dc.contributor.authorFarina, Julia Inés-
dc.contributor.authorOliveira-Junior, Sérgio Dantas-
dc.contributor.authorSales-Campos, Ceci-
dc.contributor.authorChevreuil, Larissa Ramos-
dc.date.accessioned2023-06-19T15:15:44Z-
dc.date.available2023-06-19T15:15:44Z-
dc.date.issued2023-
dc.identifier.issn16784375-
dc.identifier.urihttps://repositorio.inpa.gov.br/handle/1/39547-
dc.description.abstractGanoderma lucidum is a medicinal mushroom widely recognized as a source of biomolecules with pharmacological properties, however, little is known about the factors that influence the synthesis of bioactive proteins by this fungus when cultivated under submerged fermentation. The objective of this work was to evaluate the production of mycelial biomass and intracellular proteases and protease inhibitors by G. lucidum cultivated under different submerged fermentation conditions. The cultivation was carried out in a medium composed of glucose (10 or 20 g.L-1), soy peptone (2.5 or 5 g.L-1) and yeast extract (5 g.L-1), with incubation under agitation (120 rpm) and non-agitation, totaling 8 experimental conditions. Biomass production was determined from the dry weight, while glucose consumption was estimated by quantification of reducing sugars. The proteins were extracted in NaCl (0.15 M), and the protein extracts were submitted to protein quantification by the Bradford method, total proteolytic activity using azocasein, caseinolytic and fibrinolytic activity in Petri dishes, activity of serine (trypsin and chymotrypsin) and cysteine (papain) protease inhibitors. Cultivation in agitated condition showed higher biomass production with a maximum value of 7 g.L-1, in addition to higher activities of trypsin, chymotrypsin and papain inhibitors, with 154 IU.mg-1, 153 IU.mg-1 e 343 IU.mg-1 of protein, respectively. The non-agitated condition showed a greater potential for obtaining proteins, total proteases, caseinolytic and fibrinolytic enzymes, with maximum values of 433 mg.g-1 of extract, 71 U.mL-1 of extract, 63.62 mm2 and 50.27 mm2, respectively. Thus, a medium composed of soy peptone, yest extract and glucose in a 1:2:4 proportion is recommended, under agitation to produce protease inhibitors, and the non-agitated condition when the target is, mainly caseinolytic and fibrinolytic enzymes.pt_BR
dc.language.isoenpt_BR
dc.relation.ispartofVolume 83, Pages e270316pt_BR
dc.rightsAttribution-NonCommercial-NoDerivs 3.0 Brazil*
dc.rights.urihttp://creativecommons.org/licenses/by-nc-nd/3.0/br/*
dc.subjectBiomasspt_BR
dc.subjectTrypsinpt_BR
dc.subjectChymotrypsinpt_BR
dc.subjectPapainpt_BR
dc.subjectFermentationpt_BR
dc.subjectPeptide Hydrolasespt_BR
dc.subjectPeptonespt_BR
dc.subjectProtease Inhibitorspt_BR
dc.subjectReishipt_BR
dc.subjectGanoderma lucidumpt_BR
dc.titleProduction of mycelial biomass, proteases and protease inhibitors by Ganoderma lucidum under different submerged fermentation conditionspt_BR
dc.typeArtigopt_BR
dc.identifier.doi10.1590/1519-6984.270316-
dc.publisher.journalBrazilian journal of biology = Revista brasleira de biologiapt_BR
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