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Improved E, coli Erythromycin A Production Through the Application of Metabolic and Bioprocess Engineering

机译:通过代谢和生物工艺工程的应用改善大肠杆菌红霉素A的生产

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In this report, small-scale culture and bioreactor experiments were used to compare and improve the heterologous production of the antibiotic erythromycin A across a series of engineered prototype Escherichia coli strains. The original strain, termed BAPl(pBPJW130, pBPJW144, pHZT1, pHZT2, pHZT4, pGro7), was designed to allow full erythromycin A biosynthesis from the exogenous addition of propionate. This strain was then compared against two alternatives hypothesized to increase final product titer. Strain TB3(pBPJW130, pBPJW144, Phzt1, pHZT2, pHZT4, pGro7) is a derivative of BAP1 designed to increase biosynthetic pathway carbon flow as a result of a ygfH deletion; whereas, strain TB3(pBPJW130, pBPJW144, pHZTl, pHZT2, pHZT4-2, pGro7) provided an extra copy of a key deoxy sugar glycosyltransferase gene. Production was compared across the three strains with TB3(pBPJW130, pBPJW144, pHZT1, pHZT1, pHZT4, pGro7) showing significant improvement in erythronolide B (EB), 3-mycarosylerythronolide B (MEB), and erythromycin A titers. This strain was further tested in the context of batch bioreactor production experiments with time-course titers leveling at 4 mg/L, representing an approximately sevenfold increase in final erythromycin A titer.
机译:在本报告中,小规模的培养和生物反应器实验被用来比较和改善一系列工程原型大肠杆菌菌株中红霉素A的异源生产。最初的菌株称为BAP1(pBPJW130,pBPJW144,pHZT1,pHZT2,pHZT4,pGro7),旨在通过外源添加丙酸酯进行全红霉素A的生物合成。然后将该菌株与假设增加最终产品效价的两个替代品进行比较。菌株TB3(pBPJW130,pBPJW144,Phzt1,pHZT2,pHZT4,pGro7)是BAP1的衍生物,旨在通过ygfH缺失来增加生物合成途径的碳流量;然而,菌株TB3(pBPJW130,pBPJW144,pHZT1,pHZT2,pHZT4-2,pGro7)提供了关键脱氧糖糖基转移酶基因的额外拷贝。比较了三株TB3的产量(pBPJW130,pBPJW144,pHZT1,pHZT1,pHZT4,pGro7),显示了赤藓醇内酯B(EB),3-myososylerythronolide B(MEB)和红霉素A效价显着提高。在分批生物反应器生产实验中对该菌株进行了进一步测试,其时程滴度水平为4 mg / L,表示最终红霉素A滴度增加了约7倍。

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