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Production of rebaudioside D from stevioside using a UGTSL2 Asn358Phe mutant in a multi‐enzyme system

机译:在多酶系统中使用UGTSL2ASN358phe突变体从甜菊酰胺中生产Rebaudioside d

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Summary Rebaudioside D is a sweetener from Stevia rebaudiana with superior sweetness and organoleptic properties, but its production is limited by its minute abundance in S.?rebaudiana leaves. In this study, we established a multi‐enzyme reaction system with S.?rebaudiana UDP‐glycosyltransferases UGT76G1, Solanum lycopersicum UGTSL2 and Solanum tuberosum sucrose synthase StSUS1, achieving a two‐step glycosylation of stevioside to produce rebaudioside D. However, an increase in the accumulation of rebaudioside D required the optimization of UGTSL2 catalytic activity towards glucosylation of rebaudioside A and reducing the formation of the side‐product rebaudioside M2. On the basis of homology modelling and structural analysis, Asn358 in UGTSL2 was subjected to saturating mutagenesis, and the Asn358Phe mutant was used instead of wild‐type UGTSL2 for bioconversion. The established multi‐enzyme reaction system employing the Asn358Phe mutant produced 14.4?g?l?1 (1.6 times of wild‐type UGTSL2) rebaudioside D from 20?g?l?1 stevioside after reaction for 24?h. This system is useful for large‐scale rebaudioside D production and expands our understanding of the pathways involved in its synthesis.
机译:摘要Rebaudioside D是来自甜叶菊雷吉尼亚州的甜味剂,具有卓越的甜味和感官特性,但其生产在S.?Rebaudiana叶子中的微小丰富。在这项研究中,我们建立了一种具有S.?Rebaudiana UDP-糖基转移酶UGT76G1,Solanum Lycopersicum UGTSL2和Solanum Tuberosum蔗糖合成酶STSUS1的多酶反应体系,实现了甜菊甙的两步糖基化,以产生Rebaudioside D.然而,增加Rebaudioside D的积累所要求优化UGTSL2催化活性对莱鲍迪甙A的葡萄糖化,并减少侧面产品Rebaudioside M2的形成。在同源性建模和结构分析的基础上,对UGTSL2的ASN358进行饱和诱变,使用ASN358phe突变体代替野生型UGTSL2进行生物转化。采用ASN358phe突变体的已建立的多酶反应体系产生14.4μm≤1?1(野生型UGTSL2的1.6次)rebaudioside d从20?g?l?1甜寡在反应后24μl。该系统可用于大规模莱鲍迪甙D生产,并扩大了我们对其合成中涉及的途径的理解。

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