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糖基合成酶比色法测定的建立。

Development of a colourimetric assay for glycosynthases.

机构信息

Heinrich-Heine-Universität Düsseldorf, Institut für Bioorganische Chemie im Forschungszentrum Jülich, Gebäude: 15.8, 52426 Jülich, Germany.

Forschungszentrum Jülich, IBG-1: Biotechnology, 52425 Jülich, Germany.

出版信息

J Biotechnol. 2017 Sep 10;257:162-170. doi: 10.1016/j.jbiotec.2017.02.005. Epub 2017 Feb 11.

Abstract

The synthesis of glycosidic structures by catalysis via glycosynthases has gained much interest due to the potential high product yields and specificity of the enzymes. Nevertheless, the characterisation and implementation of new glycosynthases is greatly hampered by the lack of high-throughput methods for reaction analysis and screening of potential glycosynthase variants. Fluoride detection, via silyl ether chemosensors, has recently shown high potential for the identification of glycosynthase mutants in a high-throughput manner, though limited by the low maximal detection concentration. In the present paper, we describe a new version of a glycosynthase activity assay using a silyl ether of p-nitrophenol, allowing fast reliable detection of fluoride even at concentrations of 4mM and higher. This improvement of detection allows not only screening and identification but also kinetic characterisation of glycosynthases and synthetic reactions in a fast microtiter plate format. The applicability of the assay was successfully demonstrated by the biochemical characterisation of the mesophilic β-glucosynthase of Abg-E358S (Rhizobium radiobacter) and psychrotolerant β-glucosynthase BglU-E377A (Micrococcus antarcticus). The limitation of hyperthermophilic glycosidases as potential glycosynthases, when using glycosyl fluoride donors, was also illustrated by the example of the putative β-galactosidase GalPf from Pyrococcus furiosus.

摘要

由于酶的潜在高产物产率和特异性,通过糖基合成酶的催化合成糖苷结构引起了广泛关注。然而,新糖基合成酶的表征和实施受到缺乏用于反应分析和筛选潜在糖基合成酶变体的高通量方法的严重阻碍。最近,通过硅醚化学传感器检测氟化物,已显示出用于高通量鉴定糖基合成酶突变体的高潜力,尽管受低最大检测浓度的限制。在本文中,我们描述了一种使用对硝基苯酚硅醚的新糖基合成酶活性测定方法,即使在 4mM 及更高浓度下,也能快速可靠地检测氟化物。这种检测方法的改进不仅允许筛选和鉴定,还允许在快速微量板格式下对糖基合成酶和合成反应进行动力学表征。该测定方法的适用性通过嗜中温β-葡萄糖基合成酶 Abg-E358S(根瘤菌)和耐冷β-葡萄糖基合成酶 BglU-E377A(南极微球菌)的生化特性得到了成功证明。使用糖基氟化物供体时,嗜热糖苷酶作为潜在糖基合成酶的局限性也通过来自 Pyrococcus furiosus 的假定β-半乳糖苷酶 GalPf 的例子得到了说明。

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