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http://dx.doi.org/10.4014/jmb.1202.02020

Cloning of Agarase Gene from Non-Marine Agarolytic Bacterium Cellvibrio sp.  

Ariga, Osamu (School of Environmental Science and Engineering, Kochi University of Technology)
Inoue, Takayoshi (School of Environmental Science and Engineering, Kochi University of Technology)
Kubo, Hajime (School of Environmental Science and Engineering, Kochi University of Technology)
Minami, Kimi (School of Environmental Science and Engineering, Kochi University of Technology)
Nakamura, Mitsuteru (School of Environmental Science and Engineering, Kochi University of Technology)
Iwai, Michi (School of Environmental Science and Engineering, Kochi University of Technology)
Moriyama, Hironori (Kochi Prefectural Industrial Technology Center)
Yanagisawa, Mitsunori (International Development Engineering, Graduate School of Engineering, Tokyo Institute of Technology)
Nakasaki, Kiyohiko (International Development Engineering, Graduate School of Engineering, Tokyo Institute of Technology)
Publication Information
Journal of Microbiology and Biotechnology / v.22, no.9, 2012 , pp. 1237-1244 More about this Journal
Abstract
Agarase genes of non-marine agarolytic bacterium Cellvibrio sp. were cloned into Escherichia coli and one of the genes obtained using HindIII was sequenced. From nucleotide and putative amino acid sequences (713 aa, molecular mass; 78,771 Da) of the gene, designated as agarase AgaA, the gene was found to have closest homology to the Saccharophagus degradans (formerly, Microbulbifer degradans) 2-40 aga86 gene, belonging to glycoside hydrolase family 86 (GH86). The putative protein appears to be a non-secreted protein because of the absence of a signal sequence. The recombinant protein was purified with anion exchange and gel filtration columns after ammonium sulfate precipitation and the molecular mass (79 kDa) determined by SDS-PAGE and subsequent enzymography agreed with the estimated value, suggesting that the enzyme is monomeric. The optimal pH and temperature for enzymatic hydrolysis of agarose were 6.5 and $42.5^{\circ}C$, and the enzyme was stable under $40^{\circ}C$. LC-MS and NMR analyses revealed production of a neoagarobiose and a neoagarotetraose with a small amount of a neoagarohexaose during hydrolysis of agarose, indicating that the enzyme is a ${\beta}$-agarase.
Keywords
${\beta}$-Agarase; cloning; Cellvibrio sp.; neoagaro-oligosaccharide;
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