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http://dx.doi.org/10.5352/JLS.2009.19.4.457

Optimization of an Extracellular Dextranase Production from Lipomyces starkeyi KCTC 17343 and Analysis of Its Dextran Hydrolysates  

Chang, Yoon-Hyuck (Food Research Program, Agriculture and Agri-Food Canada)
Yeom, Joong-Hyun (Department of Oriental Medicine and Food Biotechnology, Joongbu University)
Jung, Kyung-Hwan (Department of Food and Biotechnology, Chungju University)
Chang, Byung-Chul (Department of Medical Genetic Engineering, Keimyung University School of Medicine and Institute for Medical Science)
Shin, Jung-Hee (Department of Food and Nutrition, Joongbu University)
Yoo, Sun-Kyun (Department of Oriental Medicine and Food Biotechnology, Joongbu University)
Publication Information
Journal of Life Science / v.19, no.4, 2009 , pp. 457-461 More about this Journal
Abstract
We optimized dextranase culture conditions by batch fermentation using Lipomyces starkeyi KCTC 17343. Furthermore, dextranase was purified by an ultra-membrane, and then dextran hydrolyzates were characterized. Cell growth and dextranase production varied depending on the initial culture pH and temperature. The conditions of optimal dextranase production were met in a pH range of 4-5 and temperature between $25-30^{\circ}C$. At optimal fermentation conditions, total enzyme activity and specific enzyme activity were about 4.85 IU/ml and 0.79 IU/g cells, respectively. The specific growth rate was examined to be $0.076\;hr^{-1}$. The production of dextranase in culture broth was very stably maintained after mid-log phase of growth. The enzyme hydrolyzed dextran into DP (degree of polymerization) 2 to 8 oligodextran series. Analysis of the composition of hydrolysates suggested that the enzyme produced is an endo-dextranase.
Keywords
Lipomyces starkeyi; dextranase; dextran; fermentation; oligodextran;
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