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Transcriptome analysis in mammalian cell culture: Applications in process development and characterization.

机译:哺乳动物细胞培养物中的转录组分析:在过程开发和表征中的应用。

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摘要

The advent of recombinant protein therapeutics more than two decades ago fundamentally transformed healthcare paradigms and has since improved the quality of life of millions of people. The production of these complex products is typically carried out in cultured mammalian cell lines, with a few cell lines accounting for the majority of production. Chief among these is the Chinese hamster ovary (CHO) cell line. Despite its importance, little genomic information is currently available in the public domain for this cell line. Consequently, our lab has devoted significant efforts to the development of genomic tools for CHO, including custom Affymetrix microarrays. These tools enable the global study of cellular gene expression. This thesis research has applied these transcriptome analysis tools to further understand the process of recombinant protein production.;The course of bringing a recombinant protein product to production scale involves a series of complex and often lengthy steps. As demand for these products continues to increase, there is a need to streamline process development efforts. One approach to facilitate this process is to increase our fundamental understanding of cell culture processes. Microarrays are well-suited to this application, and in this work, transcriptome analysis has been use to characterize multiple facets of cell culture process development, including cell line development and modulation of process parameters in fed-batch cultures. We found significant variation amongst clonal gene expression profiles during cell line development, an observation which could be exploited to develop gene expression-based clone screening protocols. We also uncovered the widespread impact process parameters can have on cellular gene expression. In particular, we found that raw material source, namely different hydrolysate lots, has a profound effect on the transcriptional signatures of fed-batch cell culture processes.;As next-generation sequencing technologies become increasingly mature and cost-effective, they are now being applied to the study of gene expression. We have used ultra high-throughput sequencing to investigate the deep transcriptome of CHO cells. We found that the technology correlated well with microarrays, and displayed a significantly broader detection range. Through this analysis, we also identified a number of transcriptionally-active regions in the CHO genome. The unprecedented depth achievable through next-generation sequencing now allows us to set genome sequencing firmly in our sights.
机译:二十多年前,重组蛋白疗法的问世从根本上改变了医疗模式,并从此改善了数百万人的生活质量。这些复杂产品的生产通常在培养的哺乳动物细胞系中进行,其中少数细胞系占大多数。其中最主要的是中国仓鼠卵巢(CHO)细胞系。尽管其重要性,目前在公共领域中几乎没有该细胞系的基因组信息。因此,我们的实验室投入了大量精力来开发用于CHO的基因组工具,包括定制的Affymetrix微阵列。这些工具使细胞基因表达的全球研究成为可能。本论文的研究运用了这些转录组分析工具,进一步了解了重组蛋白的生产过程。将重组蛋白产品推向生产规模的过程涉及一系列复杂且通常很长的步骤。随着对这些产品的需求持续增长,需要简化工艺开发工作。促进此过程的一种方法是增加我们对细胞培养过程的基本了解。微阵列非常适合该应用,并且在这项工作中,转录组分析已用于表征细胞培养过程发展的多个方面,包括细胞系发展和分批补料培养中过程参数的调节。我们发现细胞系发育过程中克隆基因表达谱之间存在显着差异,这一发现可用于开发基于基因表达的克隆筛选方案。我们还发现了参数对细胞基因表达的广泛影响。特别是,我们发现原材料来源(即不同批次的水解产物)对补料分批细胞培养过程的转录特征具有深远的影响。随着下一代测序技术的日益成熟和经济高效,它们正在被使用应用于基因表达的研究。我们已经使用超高通量测序来研究CHO细胞的深转录组。我们发现该技术与微阵列具有很好的相关性,并且显示出明显更宽的检测范围。通过此分析,我们还确定了CHO基因组中的许多转录活性区域。现在,通过下一代测序可获得前所未有的深度,这使我们能够坚定地设置基因组测序。

著录项

  • 作者

    Kantardjieff, Anne.;

  • 作者单位

    University of Minnesota.;

  • 授予单位 University of Minnesota.;
  • 学科 Engineering Chemical.
  • 学位 Ph.D.
  • 年度 2009
  • 页码 225 p.
  • 总页数 225
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

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