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dc.contributor.authorNisha Rani, D-
dc.contributor.authorEmilia Abraham, T-
dc.date.accessioned2015-08-15T15:07:04Z-
dc.date.available2015-08-15T15:07:04Z-
dc.date.issued2006-
dc.identifier.citationApplied Biochemistry and Biotechnology 128(3):215-226;March 2006en_US
dc.identifier.issn0273-2289-
dc.identifier.urihttp://ir.niist.res.in:8080/jspui/handle/123456789/1978-
dc.description.abstractThe Eupatorium odoratum leaf peroxidase exists as at least seven distinct isozymes (three cationic, three anionic, and one neutral). These isozymes were identified and separated by preparative iso-electric focusing. Thermal stability, including the activation enthalpy (Delta H*), free energy of inactivation (Delta G*) and activation entropy (Delta S*), and kinetic studies of two isozymes, one having a pI of 5.0 (E5) and another one having a pI of 7.0 (E7) with mol mass of 43 and 50 kD, respectively, were studied in detail. Of the molecular weight of E5 and E7, 25 and 32% correspond to the carbohydrate content of the isozymes. Optimal pH was in the acidic range of 3.6-3.8 for E5 and 3.8 for E7 with the oxidation of ABTS. E7 and E5 showed activation energy for inactivation, 194.8 and 145.4 kJ/mol, respectively. Both the isozymes showed distinct substrate specificity. The catalytic specificity constant for E5 and E7 were 112 x 105 and 124 x 10(5)/s(.)M, respectively, when 2,2'-azino-bis-(3-ethylbenz-thiazoline-6 sulfonic acid) was used as the substrate. Maximum affinity (i.e., lowest K(m) value) to H(2)O(2) was shown by E5 and E7 along with Pyrogallol and was 0.02 and 0.05/s(.)M, respectively.en_US
dc.language.isoenen_US
dc.publisherHumana Pressen_US
dc.subjectArrhenius equationen_US
dc.subjectEupatorium odoratumen_US
dc.subjectKineticsen_US
dc.subjectPeroxidaseen_US
dc.subjectThermal stabilityen_US
dc.titleKinetics and thermal stability of two peroxidase isozymes from Eupatorium odoratumen_US
dc.typeArticleen_US
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