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Bioreactor Environment-Sensitive Sentinel Genes as Novel Metrics for Cell Culture Scale-Down Comparability

机译:生物反应器环境敏感的前哨基因作为细胞培养物按比例缩小可比性的新指标。

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Scale-down of bioreactors is currently done based on matching one or more measurable parameters such as k_La and P/V, which could result in insufficient process comparability. Currently, there is a lack of genomic translational studies in cell culture scale-down, which could help delineate measurable cellular attributes for improved scale-down. In this study, we scaled-down from a typical bench-scale 5-L bioreactor to a novel high-throughput 35-mL minibioreactor based on matching oxygen transfer rate, which resulted in cell growth and product-related discrepancies using Sp2/0 cells. Performing DNA microarrays on time-course samples from both systems, we identified ~200 differentially expressed transcripts, presumably because of bioreactor aeration and mixing differences with scale-down. Evaluating these transcripts for bioreactor-relevant cellular functions such as oxidative stress response and DNA damage response, we chose 18 sentinel genes based on their degree of difference and functionality, which we further verified by quantitative real-time polymerase chain reaction (qRT-PCR). Tracking the differential expression of'Sodl, Apexl, and Odd genes, we were able to correlate sparging-related damage and poor mixing, as possible causes for physiological changes such as prolonged culture in minibioreactors. Additionally, to verify our sentinel gene findings, we performed follow-up improved scale-down studies based on gene analysis and measured transcriptomic changes. As a result, qRT-PCR-based genomic profiles and cell growth profiles showed better convergence between the improved minibioreactor conditions and the model 5-L bioreactor. Our results broadly show that based on the knowledge from transcriptomic changes of sentinel gene profiles, it is possible to improve bioreactor scale-down for more comparable processes.
机译:目前,基于匹配一个或多个可测量参数(例如k_La和P / V)来完成生物反应器的按比例缩小,这可能导致过程可比性不足。当前,缺乏在细胞培养物中按比例缩小的基因组翻译研究,这可能有助于描述可测量的细胞特性以改善按比例缩小。在这项研究中,我们根据匹配的氧气传输速率将典型的台式5升生物反应器缩减为新型高通量35毫升微型生物反应器,从而导致细胞生长和使用Sp2 / 0细胞的产物相关差异。在两个系统的时程样品上进行DNA微阵列分析,我们发现了约200个差异表达的转录本,大概是由于生物反应器通气以及比例缩小导致的混合差异。通过评估这些转录本的生物反应器相关细胞功能(例如氧化应激反应和DNA损伤反应),我们基于其差异程度和功能选择了18个前哨基因,并通过定量实时聚合酶链反应(qRT-PCR)进行了进一步验证。跟踪'Sodl,Apexl和Odd基因的差异表达,我们能够关联与喷射相关的损伤和不良的混合,这可能是造成生理变化的原因,例如微型生物反应器中长时间的培养。此外,为了验证我们的前哨基因发现,我们基于基因分析和测量的转录组学变化进行了后续改进的按比例缩小研究。结果,基于qRT-PCR的基因组图谱和细胞生长图谱显示,改进的微型生物反应器条件与模型5-L生物反应器之间具有更好的收敛性。我们的结果广泛地表明,基于前哨基因概况的转录组变化的知识,可以为更可比的过程改善生物反应器的按比例缩小。

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