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Direct measurements of IPTG enable analysis of the induction behavior of E. coli in high cell density cultures

机译:IPTG的直接测量能够分析高细胞密度培养物中大肠杆菌的诱导行为

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Background The E. coli lac operon and its components have been studied for decades, and lac-derived systems are widely used for recombinant protein production. However, lac operon dynamics and induction behavior remain the paradigm of gene regulation. Recently, an HPLC-MS-based method to quantify IPTG in the medium and inside the biomass has been established, and this tool may be useful to uncover the lack of knowledge and allow optimization of biotechnological processes. Results The results obtained from the study of IPTG distribution profiles in fed-batch, high cell density cultures allowed discrimination between two different depletion patterns of an inducer from the medium to the biomass in E. coli-expressing rhamnulose-1-phosphate aldolase (RhuA). Moreover, we could demonstrate that active transport mediates the uptake of this gratuitous inducer. Additionally, we could study the induction behaviors of this expression system by taking into account the biomass concentration at the induction time. Conclusions In the bistable range, partial induction occurred, which led to intermediate levels of RhuA activity. There was a direct relationship between the initial inducer concentrations and the initial inducer transport rate together with the specific activity. A majority of the inducer remains in the medium to reach equilibrium with the intracellular level. The intracellular inducer accumulation was a further evidence of bistability of the lac operon.
机译:背景技术大肠杆菌lac操纵子及其组件已被研究了数十年,并且lac衍生的系统被广泛用于重组蛋白的生产。然而,紫胶操纵子动力学和诱导行为仍然是基因调控的范式。最近,已经建立了一种基于HPLC-MS的方法来定量培养基中和生物质内部的IPTG,该工具可能有助于发现知识不足并优化生物技术过程。结果通过在补料分批,高细胞密度培养物中IPTG分布图的研究中获得的结果可以区分表达大肠杆菌的鼠李糖1-磷酸鼠李糖醛缩醛酶(RhuA)的两种不同的诱导剂耗尽模式,从介质到生物质。 )。此外,我们可以证明主动转运介导了这种免费诱导物的摄取。另外,我们可以通过考虑诱导时间的生物质浓度来研究该表达系统的诱导行为。结论在双稳态范围内,发生部分诱导,导致RhuA活性处于中等水平。初始诱导剂浓度和初始诱导剂转运速率与比活性之间存在直接关系。大多数诱导物保留在培养基中以达到细胞内水平的平衡。细胞内诱导剂的积累是紫胶操纵子双稳性的进一步证据。

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