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甘草黄酮类化合物途径中 UGTs 的分子克隆与功能表征。

Molecular cloning and functional characterization of UGTs from Glycyrrhiza uralensis flavonoid pathway.

机构信息

School of Chinese Materia Medica, Beijing University of Chinese Medicine, Beijing 100102, China.

School of Chinese Materia Medica, Beijing University of Chinese Medicine, Beijing 100102, China.

出版信息

Int J Biol Macromol. 2021 Dec 1;192:1108-1116. doi: 10.1016/j.ijbiomac.2021.09.136. Epub 2021 Sep 25.

DOI:10.1016/j.ijbiomac.2021.09.136
PMID:34582913
Abstract

Glycyrrhiza uralensis Fisch., a well-known medicinal plant, contains flavonoids including liquiritigenin and isoliquiritigenin, and their corresponding glycoside liquiritin and isoliquiritin. Although some genes encoding UDP-glycosyltransferases (UGTs) have been functionally characterized in G. uralensis, other UGTs mechanisms of glycosylation remain to be elucidated. Against this background the aim of the present study included cloning and characterization of two full-length cDNA clones of GuUGT isoforms from the UGT multigene family. These included GuUGT2 (NCBI acc. MK341791) and GuUGT3 (NCBI acc. MK341793) with an ORF of 1473 and 1332 bp, respectively. Multiple alignments and phylogenetic analysis revealed GuUGTs protein of Glycine max had a high homology to that of other plants. Meanwhile, quantitative real-time PCR was performed to detect the transcript levels of GuUGTs in different tissues. The results indicated that GuUGTs was more expressed in roots as compared to the leaves, and significantly up-regulated upon NaCl stress. The recombinant protein was heterologous expressed in Escherichia coli and exhibited a high level of UGT activity, catalyzing formation of isoliquiritin and liquiritin from isoliquiritigenin and liquiritigenin. The key residues of GuUGT2 for liquiritigenin glycosylation (Asn223), isoliquiritigenin (Asp272) were predicted by molecular docking and residue scanning based on simulated mutations. These results could serve as an important reference to understand the function of the UGT family. In addition, the identification of GuUGT2 and GuUGT3 provides a foundation for future studies of flavonoid biosynthesis in G. uralensis.

摘要

甘草,一种广为人知的药用植物,含有黄酮类化合物,包括甘草素和异甘草素,以及它们相应的糖苷甘草苷和异甘草苷。虽然已经对甘草中的一些编码 UDP-糖基转移酶(UGTs)的基因进行了功能表征,但其他 UGT 糖基化机制仍有待阐明。在此背景下,本研究的目的包括从 UGT 多基因家族中克隆和表征两个全长 cDNA 克隆的甘草 UGT 同工型。这些包括 GuUGT2(NCBI acc. MK341791)和 GuUGT3(NCBI acc. MK341793),其 ORF 分别为 1473 和 1332 bp。多重比对和系统发育分析表明,大豆 GuUGT 蛋白与其他植物的蛋白具有高度同源性。同时,进行了定量实时 PCR 以检测不同组织中 GuUGTs 的转录水平。结果表明,与叶片相比,GuUGTs 在根部的表达更为丰富,并且在 NaCl 胁迫下显著上调。重组蛋白在大肠杆菌中异源表达并表现出高水平的 UGT 活性,可催化异甘草素和甘草素从异甘草素和甘草素形成。通过分子对接和基于模拟突变的残基扫描预测了 GuUGT2 对甘草素糖基化(Asn223)、异甘草素(Asp272)的关键残基。这些结果可以为理解 UGT 家族的功能提供重要参考。此外,GuUGT2 和 GuUGT3 的鉴定为未来甘草黄酮类生物合成的研究提供了基础。

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