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首页> 外文期刊>Applied biochemistry and biotechnology, Part A. enzyme engineering and biotechnology >Coexpression of the Pyrroloquinoline Quinone and Glucose Dehydrogenase Genes from Serratia marcescens CTM 50650 Conferred High Mineral Phosphate-Solubilizing Ability to Escherichia coli
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Coexpression of the Pyrroloquinoline Quinone and Glucose Dehydrogenase Genes from Serratia marcescens CTM 50650 Conferred High Mineral Phosphate-Solubilizing Ability to Escherichia coli

机译:粘质沙雷氏菌CTM 50650的吡咯并喹啉醌和葡萄糖脱氢酶基因的共表达赋予大肠杆菌高矿物质磷酸盐溶解能力

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摘要

The genes gdh and pqqABCDE encoding glucose dehydrogenase and its pyrroloquinoline quinone cofactor were cloned from the mineral phosphate-solubilizing (MPS) bacterium Serratia marcescens CTM 50650.We investigated, for the first time, the impact of their coexpression in Escherichia coli on MPS ability. The production of recombinant PQQGDH conferred high MPS activity to the engineered E. coli. In fact, the amounts of soluble phosphorus (P) produced from tricalcium phosphate, hydroxyapatite, and Gafsa rock phosphate (GRP) were 574, 426, and 217 mg/L, respectively. In an attempt to increase the soluble P concentration, the E. coli strain coexpressing the gdh and pqqABCDE genes was immobilized in agar, calcium alginate, and k-carrageenan and was then further applied in a repeated batch (six batches) fermentation process to solubilize GRP. Compared to other encapsulated systems, alginate cell beads were noted to yield the highest concentration of soluble P,which attained 300mg/L/batch.MPS efficiency was maximal in the presence of 5 and 40 g/L of GRP and glucose, respectively.
机译:从溶化矿物磷酸盐的细菌Serratia marcescens CTM 50650中克隆了编码葡萄糖脱氢酶的gdh和pqqABCDE基因及其吡咯并喹啉醌辅因子,我们首次研究了它们在大肠杆菌中共表达对MPS能力的影响。重组PQQGDH的生产赋予了工程化的大肠杆菌高的MPS活性。实际上,由磷酸三钙,羟基磷灰石和磷酸加夫萨岩(GRP)产生的可溶性磷(P)的量分别为574、426和217 mg / L。为了增加可溶性P的浓度,将共表达gdh和pqqABCDE基因的大肠杆菌菌株固定在琼脂,藻酸钙和k-角叉菜胶中,然后进一步应用在重复批次(六批次)发酵过程中以使其增溶。 GRP。与其他封装系统相比,藻酸盐细胞珠产生的可溶性P浓度最高,达到300mg / L /批。当GRP和葡萄糖分别为5和40 g / L时,MPS效率最高。

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