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dc.contributor.authorDhananjay S.K
dc.contributor.authorMulimani V.H.
dc.date.accessioned2020-06-12T15:06:54Z-
dc.date.available2020-06-12T15:06:54Z-
dc.date.issued2008
dc.identifier.citationProcess Biochemistry , Vol. 43 , 6 , p. 647 - 653en_US
dc.identifier.uri10.1016/j.procbio.2008.02.010
dc.identifier.urihttp://gukir.inflibnet.ac.in:8080/jspui/handle/123456789/5325-
dc.description.abstractChitosan beads were modified with glutaraldehyde and modified chitosan was investigated as matrix for hydrophobic interaction chromatography. The influence of temperature, type of salt and its ionic strength on the adsorption of ?-galactosidase was studied. ?-Galactosidase was found to bind in presence of high concentration of ammonium sulphate (3 M, w/v) and 90% of the bound enzyme was eluted with decreasing salt concentration in presence of 10% ethylene glycol. Attempt was made to purify ?-galactosidase from modified chitosan, ?-galactosidase showed 1.7-fold purification with 43.96% recovery of enzyme activity. The SDS-PAGE analysis of enzyme showed considerable purification and its molecular weight was found to be 63-64 kDa. Unlike other chromatographic matrices, the prepared chitosan beads were used five times. The results showed that purification and recovery of the enzyme did not change even when column size was increased. © 2008 Elsevier Ltd. All rights reserved.en_US
dc.subjectAspergillus oryzae
dc.subjectChitosan
dc.subjectGlutaraldehyde
dc.subjectHydrophobic interaction chromatography
dc.subjectIonic strength
dc.subjectPurification
dc.titleEvaluation of modified chitosan as matrix for hydrophobic interaction chromatographyen_US
dc.typeArticle
Appears in Collections:1. Journal Articles

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