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新型几丁质降解菌,沙那金黄单胞菌中几丁质降解酶编码基因的分离及其编码家族 19 几丁质酶基因的特性。

Isolation of genes coding for chitin-degrading enzymes in the novel chitinolytic bacterium, Chitiniphilus shinanonensis, and characterization of a gene coding for a family 19 chitinase.

机构信息

Division of Applied Biology, Faculty of Textile Science and Technology, Shinshu University, 3-15-1 Tokida, Ueda, Nagano 386-8567, Japan.

出版信息

J Biosci Bioeng. 2012 Mar;113(3):293-9. doi: 10.1016/j.jbiosc.2011.10.018. Epub 2011 Dec 16.

Abstract

Chitiniphilus shinanonensis type strain SAY3(T) is a strongly chitinolytic bacterium, originally isolated from the moat water in Ueda, Japan. To elucidate the chitinolytic activity of this strain, 15 genes (chiA-chiO) coding for putative chitin-degrading enzymes were isolated from a genomic library. Sequence analysis revealed the genes comprised 12 family 18 chitinases, a family 19 chitinase, a family 20 β-N-acetylglucosaminidase, and a polypeptide with a chitin-binding domain but devoid of a catalytic domain. Two operons were detected among the sequences: chiCDEFG and chiLM. The gene coding for the polypeptide (chiN) showed sequence similarity to family 19 chitinases and was successfully expressed in Escherichia coli. ChiN demonstrated a multi-domain structure, composed of the N-terminal, two chitin-binding domains connected by a Pro- and Thr-rich linker, and a family 19 catalytic domain located at the C-terminus. The recombinant protein rChiN catalyzed an endo-type cleavage of N-acetyl-d-glucosamine oligomers, and also degraded insoluble chitin and soluble chitosan (degree of deacetylation of 80%). rChiN exhibited an inhibitory effect on hyphal growth of the fungus Trichoderma reesei. The chitin-binding domains of ChiN likely play an important role in the degradation of insoluble chitin, and are responsible for a growth inhibitory effect on fungi.

摘要

藤野真奈美不动杆菌模式株 SAY3(T) 是一种强烈的几丁质分解菌,最初从日本上田的护城河水中分离得到。为了阐明该菌株的几丁质分解活性,从基因组文库中分离出编码潜在几丁质降解酶的 15 个基因(chiA-chiO)。序列分析显示这些基因包括 12 个家族 18 几丁质酶、1 个家族 19 几丁质酶、1 个家族 20β-N-乙酰氨基葡萄糖苷酶和 1 个具有几丁质结合域但缺乏催化域的多肽。在这些序列中检测到两个操纵子:chiCDEFG 和 chiLM。编码该多肽(chiN)的基因与家族 19 几丁质酶具有序列相似性,并在大肠杆菌中成功表达。ChiN 表现出多结构域结构,由 N 端、通过脯氨酸和苏氨酸丰富的接头连接的两个几丁质结合域和位于 C 端的家族 19 催化结构域组成。重组蛋白 rChiN 催化 N-乙酰-d-葡萄糖胺寡聚物的内切型切割,也降解不溶性几丁质和可溶性壳聚糖(脱乙酰度为 80%)。rChiN 对真菌里氏木霉的菌丝生长表现出抑制作用。ChiN 的几丁质结合域可能在不溶性几丁质的降解中发挥重要作用,并对真菌的生长具有抑制作用。

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