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在对照和乳酸应激条件下的分批培养中,中国仓鼠卵巢细胞中 eccDNA 的微观进化动力学。

Microevolutionary dynamics of eccDNA in Chinese hamster ovary cells grown in fed-batch cultures under control and lactate-stressed conditions.

机构信息

Department of Bioengineering, Clemson University, Clemson, SC, USA.

Center for Bioinformatics and Computational Biology, University of Delaware, Newark, DE, USA.

出版信息

Sci Rep. 2023 Jan 21;13(1):1200. doi: 10.1038/s41598-023-27962-0.

Abstract

Chinese hamster ovary (CHO) cell lines are widely used to manufacture biopharmaceuticals. However, CHO cells are not an optimal expression host due to the intrinsic plasticity of the CHO genome. Genome plasticity can lead to chromosomal rearrangements, transgene exclusion, and phenotypic drift. A poorly understood genomic element of CHO cell line instability is extrachromosomal circular DNA (eccDNA) in gene expression and regulation. EccDNA can facilitate ultra-high gene expression and are found within many eukaryotes including humans, yeast, and plants. EccDNA confers genetic heterogeneity, providing selective advantages to individual cells in response to dynamic environments. In CHO cell cultures, maintaining genetic homogeneity is critical to ensuring consistent productivity and product quality. Understanding eccDNA structure, function, and microevolutionary dynamics under various culture conditions could reveal potential engineering targets for cell line optimization. In this study, eccDNA sequences were investigated at the beginning and end of two-week fed-batch cultures in an ambr250 bioreactor under control and lactate-stressed conditions. This work characterized structure and function of eccDNA in a CHO-K1 clone. Gene annotation identified 1551 unique eccDNA genes including cancer driver genes and genes involved in protein production. Furthermore, RNA-seq data is integrated to identify transcriptionally active eccDNA genes.

摘要

中国仓鼠卵巢 (CHO) 细胞系被广泛用于生产生物制药。然而,由于 CHO 基因组的固有可塑性,CHO 细胞并不是最佳的表达宿主。基因组的可塑性会导致染色体重排、转基因排除和表型漂移。CHO 细胞系不稳定性的一个尚未被充分理解的基因组元件是基因表达和调控中的染色体外环状 DNA (eccDNA)。eccDNA 可以促进超高基因表达,并且在包括人类、酵母和植物在内的许多真核生物中都有发现。eccDNA 赋予遗传异质性,为个体细胞在应对动态环境时提供了选择优势。在 CHO 细胞培养中,保持遗传同质性对于确保一致的生产力和产品质量至关重要。了解不同培养条件下 eccDNA 的结构、功能和微观进化动态可能揭示细胞系优化的潜在工程靶点。在这项研究中,在控制和乳酸盐应激条件下,在 ambr250 生物反应器中进行两周补料分批培养的开始和结束时,研究了 eccDNA 序列。本工作对 CHO-K1 克隆中的 eccDNA 结构和功能进行了表征。基因注释确定了 1551 个独特的 eccDNA 基因,包括癌症驱动基因和参与蛋白质生产的基因。此外,还整合了 RNA-seq 数据来鉴定转录活性的 eccDNA 基因。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6c49/9867765/a962239d5130/41598_2023_27962_Fig1_HTML.jpg

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