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机构地区:[1]江南大学生物工程学院糖化学与生物技术教育部重点实验室
出 处:《食品与发酵工业》2015年第8期7-11,共5页Food and Fermentation Industries
基 金:国家自然科学基金(21302069);中国博士后科学基金(2014M551500)
摘 要:将Staphylococcus carnosus来源的Fru AS.car醛缩酶基因fda和大肠杆菌来源的Yqa B磷酸酶基因yqa B分别插入到表达质粒CDFDuet-1得到重组质粒CDF-fda-yqa B,并转化该重组质粒到大肠杆菌BL21Star(DE3)。以同时过量表达Fru AS.car醛缩酶和Yqa B磷酸酶的大肠杆菌BL21Star(DE3)/CDFDuet-1-fda-yqa B作为发酵菌株,以葡萄糖为碳源通过糖酵解途径在胞内生成供体磷酸二羟基丙酮,分别在培养基中添加丙醛、丁醛为受体,进行相应稀有酮糖的合成,从而成功地将羟醛缩合反应在大肠杆菌中实现,酮糖产物用HPLC检测并进行纯化和1H NMR鉴定。最后,以13C同位素全标记的葡萄糖为碳源,添加丙醛为受体进行了同位素标记实验,证实了产物从DHAP而来的3个碳原子最终来自葡萄糖。fda gene encoding Fru AS. carfrom Staphylococcus carnosus and yqa B gene encoding Yqa B phosphatase from Escherichia coli were inserted into the expression vector CDFDuet-1 to obtain the recombinant plasmid CDF-fdayqa B. The plasmid CDF-fda-yqa B was transformed into E. coli BL21Star( DE3). The engineered E. coli BL21Star( DE3) /CDFDuet-1-fda-yqa B with capacity of co-expression of aldolase Fru AS. carand phosphatase Yqa B was used as the fermentation strain. The rare ketoses were synthesized with dihydroxyacetone phosphate( DHAP) generated in cells via glycolytic pathway as the the donor molecular and the propionaldehyde( butyraldehyde) as the acceptors.The ketose products were analyzed by HPLC and confirmed with1 H NMR after purification. In addition,the isotope experiment was performed using [U-13C6]labeled glucose as the sole carbon source with propionaldehyde as the acceptor. The result showed that C1,2,3 of the product derived from DHAP were ultimately from glucose.
分 类 号:TQ920.1[轻工技术与工程—发酵工程] Q814.9[生物学—生物工程]
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