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使用 RNA-Seq 体外监测培养的大鼠肝细胞。

Monitoring Cultured Rat Hepatocytes Using RNA-Seq In Vitro.

机构信息

Department of Biomechatronics Engineering, National Taiwan University, Taipei 106, Taiwan.

出版信息

Int J Mol Sci. 2023 Apr 19;24(8):7534. doi: 10.3390/ijms24087534.

Abstract

Compared to other techniques, RNA sequencing (RNA-Seq) has the advantage of having details of the expression abundance of all transcripts in a single run. In this study, we used RNA-Seq to monitor the maturity and dynamic characteristics of in vitro hepatocyte cultures. Hepatocytes, including mature hepatocytes and small hepatocytes, were analyzed in vitro using RNA-Seq and quantitative polymerase chain reaction (qPCR). The results demonstrated that the gene expression profiles measured by RNA-Seq showed a similar trend to the expression profiles measured by qPCR, and can be used to infer the success of in vitro hepatocyte cultures. The results of the differential analysis, which compared mature hepatocytes against small hepatocytes, revealed 836 downregulated and 137 upregulated genes. In addition, the success of the hepatocyte cultures could be explained by the gene list screened from the adopted gene enrichment test. In summary, we demonstrated that RNA-Seq could become an effective method for monitoring the whole transcriptome of hepatocyte cultures and provide a more comprehensive list of factors related to the differentiation of small hepatocytes into mature hepatocytes. This monitoring system not only shows high potential in medical applications but may also be a novel method for the clinical diagnosis of liver-related diseases.

摘要

与其他技术相比,RNA 测序 (RNA-Seq) 具有单次运行即可详细了解所有转录物表达丰度的优势。在这项研究中,我们使用 RNA-Seq 来监测体外肝细胞培养物的成熟度和动态特性。使用 RNA-Seq 和定量聚合酶链反应 (qPCR) 分析体外的肝细胞,包括成熟肝细胞和小肝细胞。结果表明,RNA-Seq 测量的基因表达谱与 qPCR 测量的表达谱具有相似的趋势,可用于推断体外肝细胞培养的成功。比较成熟肝细胞与小肝细胞的差异分析结果显示,有 836 个下调基因和 137 个上调基因。此外,通过采用基因富集试验筛选出的基因列表,可以解释肝细胞培养的成功。总之,我们证明了 RNA-Seq 可以成为监测肝细胞培养物全转录组的有效方法,并提供了与小肝细胞分化为成熟肝细胞相关的更全面的因素列表。该监测系统不仅在医学应用中具有很高的潜力,而且可能成为肝脏相关疾病临床诊断的新方法。

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