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The application of multi-parameter flow cytometry to the study of recombinant Escherichia coli batch fermentation processes

机译:多参数流式细胞术在重组大肠杆菌分批发酵过程研究中的应用

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Multi-parameter flow cytometric techniques coupled with dual colour fluorescent staining were used to study the physical and metabolic consequences of inclusion body formation in batch cultures of the recombinant Escherichia coli strain MSD3735. This strain contains a plasmid coding for the isopropylthiogalactopyranoside-inducible model eukaryotic protein AP50. It is known that the synthesis of foreign proteins at high concentrations can exert a severe metabolic stress on the host cell and that morphological changes can occur. In this work, using various points of induction, it was shown that inclusion body formation is followed immediately by measurable changes in the characteristic intrinsic light scatter patterns for the individual cell (forward scatter, 90 degrees side scatter) and a concomitant progressive change in the individual cell physiological state with respect to both cytoplasmic membrane polarisation and permeability. This work establishes flow cytometry as a potentially valuable tool for monitoring recombinant fermentation processes, providing important information for scale-up. Further, we discuss the possibility of optimising inclusion body formation by manipulating the fermentation conditions based on these rapid "real-time" measurements.
机译:多参数流式细胞仪技术结合双色荧光染色用于研究重组大肠杆菌MSD3735批培养中包涵体形成的物理和代谢后果。该菌株含有编码异丙基硫代半乳糖吡喃糖苷可诱导的模型真核蛋白AP50的质粒。众所周知,高浓度外源蛋白质的合成会在宿主细胞上施加严重的代谢应激,并且会发生形态变化。在这项工作中,利用不同的感应点,发现包涵体的形成紧随其后是单个细胞的特征固有光散射图谱的可测量变化(前向散射,90度侧向散射)以及随之而来的逐渐变化。关于细胞质膜极化和通透性的单个细胞生理状态。这项工作将流式细胞术确立为监测重组发酵过程的潜在有价值的工具,为扩大规模提供重要信息。此外,我们讨论了基于这些快速的“实时”测量值通过控制发酵条件来优化包涵体形成的可能性。

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