Biochemical characterization of dextranase from Arthrobacter oxydans and its cloning and expression in Escherichia coli

Authors :: Ghahyun J. Kim
Seong Hee Nam
Nahyun Kim
Seong-Soo Kang
Hyen Joung Park
Eun-Seong Seo
Jin-Ha Lee
Doman Kim
Young-Min Kim
Source :: Food Science and Biotechnology. 19:757-762
Publication Year :: 2010
Publisher :: Springer Science and Business Media LLC, 2010.
Abstract: Appreciably elevated levels of dextranase from Arthrobacter oxydans (AODex) isolated from sugar-cane farm soil was resulted from the culture on the Luria-Bertani (LB) medium containing 1%(w/v) soluble starch, glycerol, or dextran. The responsible gene (aodex) was cloned, its nucleotide sequence was determined, and expression of the encoded protein was achieved in Escherichia coli. An open reading frame was composed of 1,863 bp putatively encoding a 68.3 kDa protein. Recombinant A. oxydans dextranase (rAODex) was purified about 16 fold by nickel-nitrilotriacetic acid affinity column chromatography; Km value for dextran T2000 was 0.85 mg/mL (w/v). AODex treatment of stale sugar cane juice resulted in a yield of square and light-colored sugar crystals.

Subjects :: Dextranase
Nucleic acid sequence
Biology
medicine.disease_cause
Applied Microbiology and Biotechnology
law.invention
chemistry.chemical_compound
Open reading frame
chemistry
Biochemistry
Affinity chromatography
law
Glycerol
Recombinant DNA
medicine
Sugar
Escherichia coli
Food Science
Biotechnology

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