2012
DOI: 10.1590/s1517-83822012000300037
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Study on Thermodynamics and Adsorption kinetics of Purified endoglucanase (CMCase) from Penicillium notatum NCIM NO-923 produced under mixed solid-state fermentation of waste cabbage and Bagasse

Abstract: In the current study, one thermostable endoglucanase was purified from Penicillium notatum NCIM through mixed solid state fermentation of waste cabbage and bagasse. The molecular weight of the purified enzyme was 55kDa as determined by SDS polyacrylamide gel electrophoresis (SDS-PAGE). The enzyme had low activation energy (E a ) of 36.39KJ mol -1 for carboxymethyl cellulose hydrolysis and the enthalpy and entropy for irreversible inactivation was 87 kJ mol −1 and 59.3 J mol −1 K −1 respectively. The enzyme wa… Show more

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Cited by 12 publications
(5 citation statements)
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“…Increasing [P0] from 100 µg mL -1 to 263 µg mL -1 adsorption increased from 45.62 µg mL -1 to 199.0 µg mL -1 for 100 mg of Protobind as shown in Figure 18 as well. The adsorption profiles were in agreement with that of published literature [Lu et al, 2002;Chen et al, 2006;Jagar et al, 2010;Li et al, 2011;Das et al, 2012;Machado et al, 2014;Karmakar and Ray, 2015] for adsorption of enzymes on various substrates. [Baig et al, 2016] The maximum adsorption was achieved at 40 minutes of contact time.…”
Section: Adsorption Of Cellulases On Avicel and Protobindsupporting
confidence: 90%
“…Increasing [P0] from 100 µg mL -1 to 263 µg mL -1 adsorption increased from 45.62 µg mL -1 to 199.0 µg mL -1 for 100 mg of Protobind as shown in Figure 18 as well. The adsorption profiles were in agreement with that of published literature [Lu et al, 2002;Chen et al, 2006;Jagar et al, 2010;Li et al, 2011;Das et al, 2012;Machado et al, 2014;Karmakar and Ray, 2015] for adsorption of enzymes on various substrates. [Baig et al, 2016] The maximum adsorption was achieved at 40 minutes of contact time.…”
Section: Adsorption Of Cellulases On Avicel and Protobindsupporting
confidence: 90%
“…Generally, two carboxyls are involved in the catalytic mechanism of most hydrolases; one donates protons to the substrate while the other stabilizes it . Result showed the p K a1 for proton donating ionizable group and p K a2 for proton receiving residues were 2.94 and 6.53, respectively (Fig.…”
Section: Discussionmentioning
confidence: 93%
“…Dialyzed enzyme preparation was applied to a DEAE cellulose column (50 × 1 cm 2 ), pre equilibrated with buffer solution (0.05 M sodium acetate buffer; pH 5.0). The enzyme fractions were eluted with a linear gradient of 0.1–1 M NaCl at a flow rate of 0.3 ml min −1 . The fractions were collected using an auto fraction collector.…”
Section: Methodsmentioning
confidence: 99%
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