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Parallelized disruption of prokaryotic and eukaryotic cells via miniaturized and automated bead mill

机译:通过小型化和自动珠磨机并行化原核和真核细胞的破坏

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摘要

The application of integrated microbioreactor systems is rapidly becoming of more interest to accelerate strain characterization and bioprocess development. However, available high-throughput screening capabilities are often limited to target extracellular compounds only. Consequently, there is a great demand for automated technologies allowing for miniaturized and parallel cell disruption providing access to intracellular measurements. In this study, a fully automated bead mill workflow was developed and validated for four different industrial platform organisms: Escherichia coli, Corynebacterium glutamicum, Saccharomyces cerevisiae, and Aspergillus niger. The workflow enables up to 48 parallel cell disruptions in microtiter plates and is applicable at-line to running lab-scale cultivations. The resulting cell extracts form the basis for quantitative omics studies where no rapid metabolic quenching is required (e.g., genomics and proteomics).
机译:集成微生物反应器系统的应用迅速变得更加兴趣,以加速应变特征和生物过程开发。 然而,可用的高通量筛选能力通常仅限于靶细胞外化合物。 因此,对允许小型化和平行细胞破坏的自动化技术存在巨大需求,从而提供对细胞内测量的进入。 在这项研究中,为四种不同的工业平台生物体开发并验证了全自动珠轧机工作流程:大肠杆菌,玉米菌,谷氨酰胺,酿酒酵母和曲霉。 MictiroTer板上的工作流程最高可达48个平行的细胞中断,并且适用于运行实验室规模培养。 所得细胞提取物形成定量常规研究的基础,其中不需要快速代谢猝灭(例如,基因组学和蛋白质组学)。

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