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从水稻中分离出的一种缺乏参与几丁质结合的主要环结构的GH19几丁质酶的酶学性质。

Enzymatic properties of a GH19 chitinase isolated from rice lacking a major loop structure involved in chitin binding.

作者信息

Tanaka Jun, Fukamizo Tamo, Ohnuma Takayuki

机构信息

Department of Advanced Bioscience, Kindai University, 3327-204 Nakamachi, Nara 631-8505, Japan.

出版信息

Glycobiology. 2017 May 1;27(5):477-485. doi: 10.1093/glycob/cwx016.

DOI:10.1093/glycob/cwx016
PMID:28204489
Abstract

The catalytic domains of family GH19 chitinases have been found to consist of a conserved, α-helical core-region and different numbers (1-6) of loop structures, located at both ends of the substrate-binding groove and which extend over the glycon- and aglycon-binding sites. We expressed, purified and enzymatically characterized a GH19 chitinase from rice, Oryza sativa L. cv. Nipponbare (OsChia2a), lacking a major loop structure (loop III) connected to the functionally important β-stranded region. The new enzyme thus contained the five remaining loop structures (loops I, II, IV, V and C-term). The OsChia2a recombinant protein catalyzed hydrolysis of chitin oligosaccharides, (GlcNAc)n (n = 3-6), with inversion of anomeric configuration, indicating that OsChia2a correctly folded without loop III. From thermal unfolding experiments and calorimetric titrations using the inactive OsChia2a mutant (OsChia2a-E68Q), in which the catalytic residue Glu68 was mutated to glutamine, we found that the binding affinities towards (GlcNAc)n (n = 2-6) were almost proportional to the degree of polymerization of (GlcNAc)n, but were much lower than those obtained for a moss GH19 chitinase having only loop III [Ohnuma T, Sørlie M, Fukuda T, Kawamoto N, Taira T, Fukamizo T. 2011. Chitin oligosaccharide binding to a family GH19 chitinase from the moss, Bryum coronatum. FEBS J. 278:3991-4001]. Nevertheless, OsChia2a exhibited significant antifungal activity. It appears that loop III connected to the β-stranded region is important for (GlcNAc)n binding, but is not essential for antifungal activity.

摘要

已发现GH19家族几丁质酶的催化结构域由一个保守的α螺旋核心区域和不同数量(1 - 6个)的环结构组成,这些环结构位于底物结合凹槽的两端,并延伸至糖苷和糖苷配基结合位点上方。我们表达、纯化并对来自水稻日本晴(Oryza sativa L. cv. Nipponbare)的一种GH19几丁质酶(OsChia2a)进行了酶学表征,该酶缺少与功能重要的β链区域相连的一个主要环结构(环III)。因此,这种新酶包含其余五个环结构(环I、II、IV、V和C端环)。OsChia2a重组蛋白催化几丁质寡糖(GlcNAc)n(n = 3 - 6)的水解,并使异头构型发生翻转,这表明没有环III时OsChia2a也能正确折叠。通过对无活性的OsChia2a突变体(OsChia2a - E68Q,其中催化残基Glu68突变为谷氨酰胺)进行热变性实验和量热滴定,我们发现其对(GlcNAc)n(n = 2 - 6)的结合亲和力几乎与(GlcNAc)n的聚合度成正比,但远低于仅具有环III的苔藓GH19几丁质酶[大沼T,索利M,福田T,川本N,平良T,深见T。2011。几丁质寡糖与苔藓冠状真藓(Bryum coronatum)的GH19家族几丁质酶的结合。《欧洲生物化学学会联合会杂志》。278:3991 - 4001]。然而,OsChia2a表现出显著的抗真菌活性。似乎与β链区域相连的环III对(GlcNAc)n结合很重要,但对抗真菌活性并非必不可少。

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