http://www.cnr.it/ontology/cnr/individuo/prodotto/ID237690
Improvement of beta-glucodsidase activity of Olea europaea fruit extracts processed by membrane technology (Articolo in rivista)
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- Label
- Improvement of beta-glucodsidase activity of Olea europaea fruit extracts processed by membrane technology (Articolo in rivista) (literal)
- Anno
- 2006-01-01T00:00:00+01:00 (literal)
- Alternative label
R. Mazzei a, L. Giorno a, A. Spadafora b, S. Mazzuca b, E. Drioli a (2006)
Improvement of beta-glucodsidase activity of Olea europaea fruit extracts processed by membrane technology
in Korean Membrane Journal
(literal)
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- R. Mazzei a, L. Giorno a, A. Spadafora b, S. Mazzuca b, E. Drioli a (literal)
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- a ITM-CNR
b Department of Ecology, University of Calabria (literal)
- Titolo
- Improvement of beta-glucodsidase activity of Olea europaea fruit extracts processed by membrane technology (literal)
- Abstract
- The ?-glucosidase from olive fruit is of particular interest compared to the ones from other sources because
it has shown to have high specifity to convert the oleuropein into dialdehydes, which have antibacterial activity and are of
high interest for their application in the food and pharmaceutical fields. The enzyme is not yet commercially available and
advanced clean and safe technologies for its purification able to maintain the functional stability are foreseen. The purification
of this protein from fruit extracts has been already tempted by electrophoresis but either enzyme deactivation or high
background with unclear profiles occurred. In this work, fruit extracts obtained from the ripening stage that showed the
highest enzyme activity have been processed by diafiltration and ultrafiltration. Asymmetric membranes made of polyamide
or polysulphone having 50 and 30 kDa molecular weight cut-off, respectively, were tested for the diafiltration process.
Ultrafiltration membranes made of polyethersulfone with 4 kDa molecular weight cut-off were used to concentrate the diafiltered
permeate solutions. The efficiency of the separation processes was evaluated byenzyme activity tests using the hydrolysis
of p-D-nitrophenyl-?-D-glucopyranoside (pNPGlc) as reaction model. Qualitative and quantitative electrophoresis
were applied to analyze the composition of protein solution before and after the membrane separation; in addition dot blot
and western blot analyses were applied to verify the presence of ?-glucosidase in the processed fractions. The overall results
showed that the ?-glucosidase functional stability was preserved during the membrane operations and the removal of
20 kDa proteins allowed to increase the specific activity of the enzyme of about 52% compared to the one present in the
initial fruit extract. (literal)
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