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首页> 外文期刊>Journal of Biotechnology >Initial identification of low temperature and culture stage induction of miRNA expression in suspension CHO-K1 cells
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Initial identification of low temperature and culture stage induction of miRNA expression in suspension CHO-K1 cells

机译:在悬浮CHO-K1细胞中低温和培养阶段诱导miRNA表达的初步鉴定

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This paper describes the first miRNA analysis carried out on hamster cells specifically Chinese hamster ovary (CHO) cells which are the most important cell line for the manufacture of human recombinant biopharmaceutical products. During biphasic culture, an initial phase of rapid cell growth at 37 degrees C is followed by a growth arrest phase induced through reduction of the culture temperature. Growth arrest is associated with many positive phenotypes including increased productivity, sustained viability and an extended production phase. Using miRNA bioarrays generated with probes against human, mouse and rat miRNAs, we have identified 26 differentially expressed miRNAs in CHO-K1 when comparing cells undergoing exponential growth at 37 degrees C to stationary phase cells at 31 degrees C. Five miRNAs were selected for qRT-PCR analysis using specific primer sets to isolate and amplify mature miRNAs. During this analysis, two known growth inhibitory miRNAs, miR-21 and miR-24 were identified as being upregulated during stationary phase growth induced either by temperature shift or during normal batch culture by both bioarray and qRT-PCR. Sequence data confirmed the identity of cgr-miR-21, a novel Cricetulus griseus ortholog of the known miRNA miR-21. This study offers a novel insight into the potential of miRNA regulation of CHO-K1 growth and may provide novel approaches to rational engineering of both cell lines and culture processes to ensure optimal conditions for recombinant protein production.
机译:本文描述了对仓鼠细胞,特别是中国仓鼠卵巢(CHO)细胞进行的首次miRNA分析,这是制造人类重组生物药物产品最重要的细胞系。在双相培养过程中,细胞在37摄氏度快速生长的初始阶段之后是通过降低培养温度诱导的生长停滞阶段。生长停滞与许多阳性表型相关,包括提高的生产率,持续的生存能力和延长的生产阶段。使用针对人类,小鼠和大鼠miRNA的探针产生的miRNA生物阵列,当比较在37摄氏度经历指数增长的细胞与在31摄氏度经历平稳期的细胞进行比较时,我们已经在CHO-K1中鉴定出26种差异表达的miRNA。选择了5种miRNA用于qRT -PCR分析,使用特定的引物对分离和扩增成熟的miRNA。在此分析过程中,通过生物芯片和qRT-PCR鉴定出了两个已知的生长抑制性miRNA,miR-21和miR-24在温度变化诱导的稳定期生长或正常分批培养过程中被上调。序列数据证实了cgr-miR-21的身份,cgr-miR-21是已知miRNA miR-21的新型灰C直向同源物。这项研究提供了对CHO-K1生长的miRNA调控潜力的新见解,并可能为合理设计细胞系和培养过程提供新方法,以确保重组蛋白生产的最佳条件。

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