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Structural analysis of rebaudioside A derivatives obtained by Lactobacillus reuteri 180 glucansucrase-catalyzed trans-α-glucosylation

机译:罗伊氏乳杆菌180葡聚糖蔗糖酶催化反式α-葡萄糖基化反应获得莱鲍迪甙A衍生物的结构分析

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摘要

The wild-type Gtf180-ΔN glucansucrase enzyme from Lactobacillus reuteri 180 was found to catalyze the α-glucosylation of the steviol glycoside rebaudioside A, using sucrose as glucosyl donor in a transglucosylation process. Structural analysis of the formed products by MALDI-TOF mass spectrometry, methylation analysis and NMR spectroscopy showed that rebaudioside A is specifically α-d-glucosylated at the steviol C-19 β-d-glucosyl moiety (55% conversion). The main product is a mono-(α1 → 6)-glucosylated derivative (RebA-G1). A series of minor products, up to the incorporation of eight glucose residues, comprise elongations of RebA-G1 with mainly alternating (α1 → 3)- and (α1 → 6)-linked glucopyranose residues. These studies were carried out in the context of a program directed to the improvement of the taste of steviol glycosides via enzymatic modification of their naturally occurring carbohydrate moieties.
机译:发现来自罗伊氏乳杆菌180的野生型Gtf180-ΔN葡糖苷酸酶在转糖基化过程中使用蔗糖作为葡糖基供体来催化甜菊糖苷莱鲍迪苷A的α-糖基化。通过MALDI-TOF质谱,甲基化分析和NMR光谱对形成的产物进行结构分析表明,莱鲍迪甙A在甜菊糖C-19β-d-葡萄糖基部分上被α-d-葡萄糖基化(55%转化率)。主要产品是单-(α1→6)-葡萄糖基化衍生物(RebA-G1)。一系列次要产品,最多可掺入八个葡萄糖残基,包括RebA-G1的延伸,主要带有交替交替的(α1→3)-和(α1→6)连接的吡喃葡萄糖残基。这些研究是在一个程序的框架内进行的,该程序旨在通过酶促修饰天然存在的碳水化合物部分来改善甜菊糖苷的口味。

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