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用于在复杂介质中测量酶活性的多糖和含碳水化合物生物聚合物的荧光衍生化

Fluorescent derivatization of polysaccharides and carbohydrate-containing biopolymers for measurement of enzyme activities in complex media.

作者信息

Arnosti C

机构信息

Department of Marine Sciences, 12-7 Venable Hall CB #3300, University of North Carolina, Chapel Hill, NC 27599-3300, USA.

出版信息

J Chromatogr B Analyt Technol Biomed Life Sci. 2003 Aug 5;793(1):181-91. doi: 10.1016/s1570-0232(03)00375-1.

Abstract

Fluorescence derivatization provides a means of tracing the dynamics of polysaccharides even in the presence of high concentrations of other organic compounds or salts. A method of labeling polysaccharides with fluoresceinamine was extended to polysaccharides of a wide range of chemical composition, and alternative means of preparation were established for polysaccharides not initially amenable to column chromatography. The polysaccharides were activated with cyanogen bromide, coupled to fluoresceinamine, and separated from unreacted fluorophore via gel filtration chromatography or dialysis. Since the resulting derivatized polysaccharides proved to be stable to further physical and chemical manipulation, methods were also developed for re-activation and labeling with a second fluorophore, as well as for tethering the labeled polysaccharides to agarose beads. As an example of the application of this approach, five distinct fluorescently-labeled polysaccharides (pullulan, laminarin, xylan, chondroitin sulfate, and alginic acid) were used to investigate the activities and structural specificities of extracellular enzymes produced in situ by marine microbial communities, providing a means of measuring specifically the activities of endo-acting extracellular enzymes and avoiding use of low molecular mass substrate proxies. These labeled polysaccharides could be used to explore the dynamics of polysaccharides in other types of complex media, as well as to investigate the activities and specificities of endo-acting enzymes in other systems.

摘要

荧光衍生化提供了一种追踪多糖动态变化的方法,即使在存在高浓度其他有机化合物或盐的情况下也能如此。一种用荧光胺标记多糖的方法被扩展到具有广泛化学组成的多糖,并且为最初不适合柱色谱的多糖建立了替代的制备方法。多糖用溴化氰活化,与荧光胺偶联,并通过凝胶过滤色谱或透析与未反应的荧光团分离。由于所得的衍生化多糖被证明对进一步的物理和化学操作稳定,还开发了用第二种荧光团重新活化和标记的方法,以及将标记的多糖连接到琼脂糖珠上的方法。作为这种方法应用的一个例子,五种不同的荧光标记多糖(支链淀粉、海带多糖、木聚糖、硫酸软骨素和海藻酸)被用于研究海洋微生物群落原位产生的细胞外酶的活性和结构特异性,提供了一种专门测量内切作用细胞外酶活性并避免使用低分子量底物替代物的方法。这些标记的多糖可用于探索其他类型复杂介质中多糖的动态变化,以及研究其他系统中内切作用酶的活性和特异性。

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