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转录组学作为评估哺乳动物细胞灌注系统可扩展性的工具。

Transcriptomics as a tool for assessing the scalability of mammalian cell perfusion systems.

机构信息

Cell Culture Development, Global Biological Development Bayer HealthCare, 800 Dwight Way, Berkeley, CA, 94710, USA.

出版信息

Adv Biochem Eng Biotechnol. 2014;139:227-43. doi: 10.1007/10_2013_239.

Abstract

DNA microarray-based transcriptomics have been used to determine the time course of laboratory and manufacturing-scale perfusion bioreactors in an attempt to characterize cell physiological state at these two bioreactor scales. Given the limited availability of genomic data for baby hamster kidney (BHK) cells, a Chinese hamster ovary (CHO)-based microarray was used following a feasibility assessment of cross-species hybridization. A heat shock experiment was performed using both BHK and CHO cells and resulting DNA microarray data were analyzed using a filtering criteria of perfect match (PM)/single base mismatch (MM) > 1.5 and PM-MM > 50 to exclude probes with low specificity or sensitivity for cross-species hybridizations. For BHK cells, 8910 probe sets (39 %) passed the cutoff criteria, whereas 12,961 probe sets (56 %) passed the cutoff criteria for CHO cells. Yet, the data from BHK cells allowed distinct clustering of heat shock and control samples as well as identification of biologically relevant genes as being differentially expressed, indicating the utility of cross-species hybridization. Subsequently, DNA microarray analysis was performed on time course samples from laboratory- and manufacturing-scale perfusion bioreactors that were operated under the same conditions. A majority of the variability (37 %) was associated with the first principal component (PC-1). Although PC-1 changed monotonically with culture duration, the trends were very similar in both the laboratory and manufacturing-scale bioreactors. Therefore, despite time-related changes to the cell physiological state, transcriptomic fingerprints were similar across the two bioreactor scales at any given instance in culture. Multiple genes were identified with time-course expression profiles that were very highly correlated (> 0.9) with bioprocess variables of interest. Although the current incomplete annotation limits the biological interpretation of these observations, their full potential may be realized in due course when richer genomic data become available. By taking a pragmatic approach of transcriptome fingerprinting, we have demonstrated the utility of systems biology to support the comparability of laboratory and manufacturing-scale perfusion systems. Scale-down model qualification is the first step in process characterization and hence is an integral component of robust regulatory filings. Augmenting the current paradigm, which relies primarily on cell culture and product quality information, with gene expression data can help make a substantially stronger case for similarity. With continued advances in systems biology approaches, we expect them to be seamlessly integrated into bioprocess development, which can translate into more robust and high yielding processes that can ultimately reduce cost of care for patients.

摘要

基于 DNA 微阵列的转录组学已被用于确定实验室和制造规模灌注生物反应器的时间过程,试图在这两个生物反应器规模上描述细胞的生理状态。鉴于仓鼠肾(BHK)细胞的基因组数据有限,在对种间杂交进行可行性评估后,使用了基于中国仓鼠卵巢(CHO)的微阵列。对 BHK 和 CHO 细胞进行了热休克实验,并用完美匹配(PM)/单碱基错配(MM)>1.5 和 PM-MM>50 的过滤标准分析所得 DNA 微阵列数据,以排除种间杂交特异性或敏感性低的探针。对于 BHK 细胞,8910 个探针集(39%)通过了截止标准,而对于 CHO 细胞,12961 个探针集(56%)通过了截止标准。然而,BHK 细胞的数据允许热休克和对照样品的明显聚类以及鉴定出具有差异表达的生物学相关基因,表明种间杂交的实用性。随后,在相同条件下运行的实验室和制造规模灌注生物反应器的时间过程样品上进行了 DNA 微阵列分析。大部分可变性(37%)与第一主成分(PC-1)相关。尽管 PC-1 随培养时间单调变化,但在实验室和制造规模生物反应器中,趋势非常相似。因此,尽管细胞生理状态随时间发生变化,但在培养过程中的任何给定时间,两个生物反应器规模的转录组指纹都相似。确定了具有时间过程表达谱的多个基因,这些基因与感兴趣的生物过程变量高度相关(>0.9)。尽管当前不完整的注释限制了对这些观察结果的生物学解释,但随着更丰富的基因组数据的出现,它们的全部潜力可能会在适当的时候实现。通过采用转录组指纹的务实方法,我们证明了系统生物学在支持实验室和制造规模灌注系统的可比性方面的实用性。缩小模型鉴定是过程特性化的第一步,因此是稳健监管申报的一个组成部分。用基因表达数据来补充当前主要依赖于细胞培养和产品质量信息的范式,可以帮助更好地证明相似性。随着系统生物学方法的不断进步,我们预计它们将无缝集成到生物过程开发中,这可以转化为更稳健和高产的过程,最终可以降低患者的治疗成本。

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