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首页> 外文期刊>Journal of industrial microbiology & biotechnology >Dextran dextrinase and dextran of Gluconobacter oxydans
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Dextran dextrinase and dextran of Gluconobacter oxydans

机译:氧化葡糖杆菌的葡聚糖糊精酶和葡聚糖

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摘要

Certain strains of Gluconobacter oxydans have been known since the 1940s to produce the enzyme dextran dextrinase (DDase; EC2.4.1.2)-a transglucosidase converting maltodextrins into (oligo)dextran. The enzyme catalyses the transfer of an alpha1,4 linked glucosyl unit from a donor to an acceptor molecule, forming an alpha1,6 linkage: consecutive glucosyl transfers result in the formation of high molecular weight dextran from maltodextrins. In the early 1990s, the group of K. Yamamoto in Japan revived research on DDase, focussing on the purification and characterisation of the intracellular DDase produced by G. oxydans ATCC 11894. More recently, this was taken further by Y. Suzuki and coworkers, who investigated the properties and kinetics of the extracellular DDase formed by the same strain. Our group further elaborated on fermentation processes to optimise DDase production and dextran formation, DDase characterisation and its use as a biocatalyst, and the physiological link between intracellular and extracellular DDase. Here, we present a condensed overview of the current scientific status and the application potential of G. oxydans DDase and its products, (oligo)dextrans. The production of DDase as well as of dextran is first described via optimised fermentation processes. Specific assays for measuring DDase activity are also outlined. The general characteristics, substrate specificity, and mode of action of DDase as a transglucosidase are described in detail. Two forms of DDase are produced by G. oxydans depending on nutritional fermentation conditions: an intracellular and an extracellular form. The relationship between the two enzyme forms is also discussed. Furthermore, applications of DDase, e.g. production of (oligo)dextran, transglucosylated products and speciality oligosaccharides, are summarized.
机译:自1940年代以来,已知某些氧化葡糖杆菌菌株会产生葡聚糖酶(DDase; EC2.4.1.2)-一种将麦芽糖糊精转化为(寡聚)葡聚糖的转葡糖苷酶。该酶催化α1,4连接的葡萄糖基单元从供体转移到受体分子,形成α1,6连接:连续的葡萄糖基转移导致麦芽糖糊精形成高分子量的葡聚糖。在1990年代初期,日本的山本K.小组恢复了对DDase的研究,重点研究了氧化羟色胺(G. oxydans)ATCC 11894产生的细胞内DDase的纯化和鉴定。他们研究了同一菌株形成的细胞外DDase的特性和动力学。我们的小组进一步阐述了发酵工艺,以优化DDase的生产和葡聚糖的形成,DDase的表征及其作为生物催化剂的用途以及细胞内和细胞外DDase之间的生理联系。在这里,我们简要概述了当前的科学现状和氧化丁香双歧杆菌DDase及其产品(寡聚)葡聚糖的应用潜力。首先通过优化的发酵过程描述DDase和葡聚糖的生产。还概述了用于测量DDase活性的特定测定法。详细描述了DDase作为转葡糖苷酶的一般特性,底物特异性和作用方式。氧化单歧杆菌根据营养发酵条件产生两种形式的DDase:细胞内和细胞外形式。还讨论了两种酶形式之间的关系。此外,DDase的应用例如总结了(低聚)右旋糖酐的生产,转糖基化产物和特种低聚糖。

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