Heat-stability and primary structure of the major alginate lyase isozyme LbAly35 from Littorina brevicula
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概要
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Previously we isolated the major alginate lyase isozyme LbAly35 from a marine snail Littorina brevicula and showed that this enzyme was significantly heat-stable in a broad pH range compared with other molluscan alginate lyases (Hata et al., Fish Sci. (2009) 75:755-763). LbAly35 showed practically no similarity to other molluscan alginate lyases in the N-terminal amino-acid sequence of 20 residues and no cross-reactivity with anti-abalone alginate lyase antiserum. These led us to consider that the primary structure of LbAly35 is considerably deviated from other molluscan enzymes. Thus, in the present study, we first compared the thermal stability of LbAly35 with an abalone alginate lyase, HdAly, and found that the first order inactivation rate constants for LbAly35 at 40℃ and 45℃ were 1/20 and 1/45 of those for HdAly, respectively. Then, we cloned cDNAs encoding LbAly35 and characterized its deduced amino-acid sequence comparing with those of other molluscan alginate lyases. The cDNAs were amplified by PCR and 5'- and 3'-RACE PCRs from the L. brevicula hepatopancreas cDNA using degenerated primers synthesized on the basis of partial amino-acid sequences of LbAly35. The cDNA covering entire translational region of LbAly35 comprised 1,093 bp and encoded an amino-acid sequence of 296 residues. The amino-acid sequence consisted of an initiation methionine, a putative signal peptide for secretion (22 residues), a propeptide-like region (10 residues), and a mature LbAly35 domain of 263 residues. Although the N-terminal region of LbAly35 was significantly deviated from those of other molluscan alginate lyases, the catalytic domain of LbAly35 showed ~45% identity to other molluscan enzymes which had been classified under polysaccharide-lyase-family-14 (PL-14). In addition, the amino-acid residues crucially important for the catalytic actions of PL-14 enzymes were also conserved in LbAly35. Accordingly, LbAly35 was regarded as a member of PL-14 as other molluscan alginate lyases despite of the significant deviation of its N-terminal region.
- 2012-07-01
著者
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Ojima Takao
Lab. Of Marine Biotechnology And Microbiology Graduate School Of Fisheries Sciences Hokkaido Univ. H
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INOUE Akira
Laboratory of Marine Biotechnology and Microbiology, Graduate School of Fisheries Sciences, Hokkaido
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Ojima Takao
Laboratory Of Biochemistry And Biotechnology Graduate School Of Fisheries Sciences Hokkaido Universi
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Rahman Mohammad
Laboratory Of Function And Morphology Department Of Animal Science Faculty Of Agriculture Utsunomiya
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Rahman Mohammad
Laboratory Of Marine Biotechnology And Microbiology Graduate School Of Fisheries Sciences Hokkaido University
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Wang Ling
Laboratory Of Marine Biotechnology And Microbiology Graduate School Of Fisheries Sciences Hokkaido University
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Inoue Akira
Laboratory Of Marine Biotechnology And Microbiology Graduate School Of Fisheries Sciences Hokkaido University
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Rahman Mohammad
Laboratory for Nanoelectronics and Spintronics, Research Institute of Electrical Communication, Tohoku University, Sendai 980-8577, Japan
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Inoue Akira
Laboratory of Biochemistry and Biotechnology, Graduate School of Fisheries Sciences, Hokkaido University
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Rahman Mohammad
Laboratory for Nanoelectronics and Spintronics, Research Institute of Electrical Communication, Tohoku University, 2-1-1 Katahira, Aoba-ku, Sendai 980-8577, Japan
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