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A barley xyloglucan xyloglucosyl transferase covalently links xyloglucan, cellulosic substrates, and (1 3;1 4)-beta-D-glucans

机译:大麦木葡聚糖木葡糖基转移酶共价连接木葡聚糖,纤维素底物和(1 3; 1 4)-β-D-葡聚糖

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摘要

Molecular interactions between wall polysaccharides, which include cellulose and a range of noncellulosic polysaccharides such as xyloglucans and (1,3;1,4)-β-d-glucans, are fundamental to cell wall properties. These interactions have been assumed to be noncovalent in nature in most cases. Here we show that a highly purified barley xyloglucan xyloglucosyl transferase HvXET5 (EC 2.4.1.207), a member of the GH16 group of glycoside hydrolases, catalyzes the in vitro formation of covalent linkages between xyloglucans and cellulosic substrates and between xyloglucans and (1,3;1,4)-β-d-glucans. The rate of covalent bond formation catalyzed by HvXET5 with hydroxyethylcellulose (HEC) is comparable with that on tamarind xyloglucan, whereas that with (1,3; 1,4)-β-d-glucan is significant but slower. Matrix-assisted laser desorption ionization time-of-flight mass spectrometric analyses showed that oligosaccharides released from the fluorescent HEC:xyloglucan conjugate by a specific (1,4)-β-dglucan endohydrolase consisted of xyloglucan substrate with one, two, or three glucosyl residues attached. Ancillary peaks contained hydroxyethyl substituents (m/z 45) and confirmed that the parent material consisted of HEC covalently linked with xyloglucan. Similarly, partial hydrolysis of the (1,3;1,4)-β-d-glucan:xyloglucan conjugate by a specific (1,3;1,4)-β-d-glucan endohydrolase revealed the presence of a series of fluorescent oligosaccharides that consisted of the fluorescent xyloglucan acceptor substrate linked covalently with 2-6 glucosyl residues. These findings raise the possibility that xyloglucan endo-transglucosylases could link different polysaccharides in vivo and hence influence cell wall strength, flexibility, and porosity.
机译:壁多糖(包括纤维素)和一系列非纤维素多糖(如木葡聚糖和(1,3; 1,4)-β-d-葡聚糖)之间的分子相互作用是细胞壁特性的基础。在大多数情况下,已假定这些相互作用本质上是非共价的。在这里我们显示了高纯度的大麦木葡聚糖葡糖基转移酶HvXET5(EC 2.4.1.207),是糖苷水解酶GH16组的成员,催化了木葡聚糖与纤维素底物之间以及木葡聚糖与(1,3之间的共价键的体外形成。 ; 1,4)-β-d-葡聚糖。 HvXET5与羟乙基纤维素(HEC)催化的共价键形成速率与罗望子木葡聚糖的速率相当,而(1,3; 1,4)-β-d-葡聚糖的速率显着,但较慢。基质辅助激光解吸电离飞行时间质谱分析表明,通过特定的(1,4)-β-d-葡聚糖内切酶从荧光HEC:木葡聚糖缀合物释放的寡糖由木葡聚糖底物和一个,两个或三个葡糖基组成残留物附着。辅助峰包含羟乙基取代基(m / z 45),并确认母体材料由与木葡聚糖共价连接的HEC组成。同样,(1,3; 1,4)-β-d-葡聚糖:木葡聚糖偶联物被特定的(1,3; 1,4)-β-d-葡聚糖内切酶部分水解显示存在一系列荧光寡糖,由荧光木糖葡聚糖受体底物与2-6个葡萄糖基残基共价连接而成。这些发现增加了木葡聚糖内转葡糖基化酶可以在体内连接不同的多糖并因此影响细胞壁强度,柔韧性和孔隙度的可能性。

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