首页> 外文期刊>Applied Microbiology and Biotechnology >Molecular cloning, purification, and characterization of a novel polyMG-specific alginate lyase responsible for alginate MG block degradation in Stenotrophomas maltophilia KJ-2
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Molecular cloning, purification, and characterization of a novel polyMG-specific alginate lyase responsible for alginate MG block degradation in Stenotrophomas maltophilia KJ-2

机译:新型聚MG特异性藻酸盐裂解酶的分子克隆,纯化和表征,负责嗜麦芽窄食单胞菌KJ-2中的藻酸盐MG阻滞降解。

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摘要

A gene for a polyMG-specific alginate lyase possessing a novel structure was identified and cloned from Stenotrophomas maltophilia KJ-2 by using PCR with homologous nucleotide sequences-based primers. The recombinant alginate lyase consisting of 475 amino acids was purified on Ni-Sepharose column and exhibited the highest activity at pH 8 and 40 °C. Interestingly, the recombinant alginate lyase was expected to have a similar catalytic active site of chondroitin B lyase but did not show chondroitin lyase activity. In the test of substrate specificity, the recombinant alginate lyase preferentially degraded the glycosidic bond of polyMG-block than polyM-block and polyG-block. The chemical structures of the degraded alginate oligosaccharides were elucidated to have mannuronate (M) at the reducing end on the basis of NMR analysis, supporting that KJ-2 polyMG-specific alginate lyase preferably degraded the glycosidic bond in M-G linkage than that in G-M linkage. The KJ-2 polyMG-specific alginate lyase can be used in combination with other alginate lyases for a synergistic saccharification of alginate.
机译:通过使用基于同源核苷酸序列的引物的PCR,鉴定了具有新颖结构的polyMG特异性藻酸盐裂解酶的基因,并从嗜麦芽窄食单胞菌KJ-2中克隆了该基因。在Ni-Sepharose柱上纯化了由475个氨基酸组成的重组藻酸盐裂解酶,并在pH 8和40°C下表现出最高的活性。有趣的是,预期重组藻酸盐裂解酶具有软骨素B裂解酶的相似催化活性位点,但不显示软骨素裂解酶活性。在底物特异性测试中,重组藻酸盐裂解酶比polyM-block和polyG-block优先降解polyMG-block的糖苷键。根据NMR分析,阐明了降解的藻酸盐寡糖的化学结构在还原端具有甘露糖酸酯(M),支持了KJ-2聚MG特异性藻酸盐裂解酶比MG链接中的糖苷键更易降解。 KJ-2 polyMG特有的藻酸盐裂解酶可与其他藻酸盐裂解酶结合使用,以协同糖化藻酸盐。

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