Cloning of a gene encoding glycosyltransferase from Pueraria lobata (Wild.) Ohwi and its expression in Pichia pastoris

被引:0
|
作者
Zhou, Wenling [1 ,2 ]
Wang, Yinghua [3 ]
Chen, Gang [3 ]
Lue, Min [1 ]
LixiaYang [1 ]
Hu, Xiaoxiang [1 ]
Li, Haihang [1 ]
Li, Ling [1 ]
机构
[1] S China Normal Univ, Guangdong Prov Key Lab Biotechnol Plant Dev, Coll Life Sci, Guangzhou 510631, Guangdong, Peoples R China
[2] Guangzhou Sugarcane Ind Res Inst, Guangzhou 510316, Guangdong, Peoples R China
[3] Zhaoqing Univ, Dept Biol, Zhaoqing 526061, Peoples R China
来源
AFRICAN JOURNAL OF BIOTECHNOLOGY | 2011年 / 10卷 / 01期
关键词
Pueraria lobata (Willd.) Ohwi; glycosyltransferase; cloning; expression; Pichia pastoris; HIGH-LEVEL EXPRESSION; SPONTANEOUSLY HYPERTENSIVE-RATS; LEGUME MEDICAGO-TRUNCATULA; B SURFACE-ANTIGEN; METHYLOTROPHIC YEAST; MOLECULAR-CLONING; FUNCTIONAL-CHARACTERIZATION; UDP-GLUCOSYLTRANSFERASE; ARABIDOPSIS-THALIANA; SALICYLIC-ACID;
D O I
暂无
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
The key enzyme of puerarin biosynthesis in Pueraria lobata (Willd.) Ohwi was unclear but may involve glycosylation. To investigate the regulation of puerarin biosynthesis, a putative UDP-dependent glycosyltransferase (UGT) gene, PlUGT1 was isolated from P. lobata root, which contained abundant puerarin. PlUGT1 encoded 480 deduced amino acid residues with a conserved UDP-glucose-binding domain, which has 61 to 84% similarity to homologues from other plant species. SDS polyacrylamide gel electrophoresis and western blotting results showed that, fusion protein migrated as a single protein band with a molecular weight of 55 kDa. A yeast expression vector pPICZA-PlUGT1 was constructed and was transformed into Pichia pastoris strain GS115. Several recombinants containing multi-copy expression cassettes were obtained on the zeocin-YPD plate and confirmed by southern dot blotting. The yield of PlUGT1 attained 0.05 g/l when recombinant cells were cultured at pH 5.5, 30 degrees C and induced with 0.5% methanol for 72 h. The expression of PlUGT1 protein correlates positively with the copy numbers of PlUGT1 in transformed yeast cells. These results suggest that, the PlUGT1 protein can be expressed efficiently in the P. pastoris expression system and may supply a new economic and convenient way for the production of PlUGT1 protein.
引用
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页码:85 / 96
页数:12
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