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通过将合成寡糖掺入植物细胞壁来分析木葡聚糖内转糖基酶。

Analyzing Xyloglucan Endotransglycosylases by Incorporating Synthetic Oligosaccharides into Plant Cell Walls.

机构信息

Department of Biomolecular Systems, Max Planck Institute of Colloids and Interfaces, Am Mühlenberg 1, 14476, Potsdam, Germany.

Freie Universität Berlin, Institute of Chemistry and Biochemistry, Arnimallee 22, 14195, Berlin, Germany.

出版信息

Chembiochem. 2018 Apr 16;19(8):793-798. doi: 10.1002/cbic.201700638. Epub 2018 Feb 23.

Abstract

The plant cell wall is a cellular exoskeleton consisting predominantly of a complex polysaccharide network that defines the shape of cells. During growth, this network can be loosened through the action of xyloglucan endotransglycosylases (XETs), glycoside hydrolases that "cut and paste" xyloglucan polysaccharides through a transglycosylation process. We have analyzed cohorts of XETs in different plant species to evaluate the substrate specificities of xyloglucan acceptors by using a set of synthetic oligosaccharides obtained by automated glycan assembly. The ability of XETs to incorporate the oligosaccharides into polysaccharides printed as microarrays and into stem sections of Arabidopsis thaliana, beans, and peas was assessed. We found that single xylose substitutions are sufficient for transfer, and xylosylation of the terminal glucose residue is not required by XETs, independent of plant species. To obtain information on the potential xylosylation pattern of the natural acceptor of XETs, that is, the nonreducing end of xyloglucan, we further tested the activity of xyloglucan xylosyl transferase (XXT) 2 on the synthetic xyloglucan oligosaccharides. These data shed light on inconsistencies between previous studies towards determining the acceptor substrate specificities of XETs and have important implications for further understanding plant cell wall polysaccharide synthesis and remodeling.

摘要

植物细胞壁是一种细胞外骨骼,主要由复杂的多糖网络组成,该网络决定了细胞的形状。在生长过程中,通过木葡聚糖内转糖基酶(XET)的作用,可以使该网络变得松散,木葡聚糖内转糖基酶是一种糖苷水解酶,通过转糖基化过程“切割和粘贴”木葡聚糖多糖。我们分析了不同植物物种中的 XET 群体,以通过使用一组通过自动糖基化组装获得的合成低聚糖来评估木葡聚糖受体的底物特异性。评估了 XET 将低聚糖掺入作为微阵列打印的多糖中和拟南芥、豆类和豌豆茎段中的能力。我们发现,单糖取代足以进行转移,并且 XET 不需要糖基化末端葡萄糖残基,而与植物物种无关。为了获得有关 XET 的天然受体(即木葡聚糖的非还原端)的潜在木糖基化模式的信息,我们进一步在合成木葡聚糖低聚糖上测试了木葡聚糖木糖基转移酶(XXT)2 的活性。这些数据阐明了先前研究确定 XET 受体底物特异性之间的不一致性,并对进一步了解植物细胞壁多糖合成和重塑具有重要意义。

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