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Regulated expression of the Alcaligenes eutrophus pha biosynthesis genes in Escherichia coli.

机译:拟南芥嗜碱生物合成基因在大肠杆菌中的调控表达。

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摘要

A novel poly-beta-hydroxybutyrate (PHB) production system in which the expression and gene dosage of the Alcaligenes eutrophus pha biosynthetic operon were effectively regulated by cultivation temperature was constructed in Escherichia coli. The pha operon was fused to the negatively regulated tac promoter and cloned into a vector in which the copy number is temperature dependent. A two-phase process was employed to produce PHB during fed-batch growth. In the growth phase, the culture was maintained at a low temperature. Under this condition, the plasmid copy number was depressed and the number of LacI proteins was sufficient to repress tacupha transcription. The production phase was initiated by temperature upshift. At the elevated temperature, the number of plasmids surpassed the number of LacI repressors, which resulted in rapid induction of tacupha transcription, synthesis of poly-beta-hydroxyalkanoate-specific proteins, and polymer synthesis. During the production phase, the PHB production rate was 1.07 g of PHB liter-1 h-1 under optimized conditions. This rate is comparable to that of bacteria which naturally produce this polymer.
机译:在大肠杆菌中构建了一种新型的聚β-羟基丁酸酯(PHB)生产系统,该系统可以通过培养温度有效地调控真人拟南芥生化因子操纵子的表达和基因剂量。将pha操纵子与负调控的tac启动子融合,并克隆到拷贝数与温度有关的载体中。在分批补料生长过程中,采用两阶段工艺生产PHB。在生长期,将培养物保持在低温下。在这种条件下,质粒拷贝数降低,LacI蛋白的数量足以抑制tacupha转录。生产阶段通过温度升高开始。在升高的温度下,质粒的数量超过了LacI阻遏物的数量,从而导致了Tacupha转录的快速诱导,聚β-羟基链烷酸酯特异性蛋白的合成以及聚合物的合成。在生产阶段,在最佳条件下,PHB的产量为1.07 g PHB升-1 h-1。该速率与天然产生这种聚合物的细菌的速率相当。

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