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Identification of Salt-Stress-Induced Genes from the RNA-Seq Data of Reaumuria trigyna Using Differential-Display Reverse Transcription PCR

机译:利用差示逆转录PCR从红砂的RNA-Seq数据鉴定盐胁迫诱导的基因

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摘要

Next generation sequencing (NGS) technologies have been used to generate huge amounts of sequencing data from many organisms. However, the correct choice of candidate genes and prevention of false-positive results computed from digital gene expression (DGE) of RNA-seq data are vital when using these genetic resources. We indirectly identified 18 salt-stress-induced Reaumuria trigyna transcripts from the transcriptome sequencing data using differential-display reverse transcription PCR (DDRT-PCR) combined with local BLAST searches. Highly consistent with the DGE results, the quantitative real-time PCR expression patterns of these transcripts showed strong upregulation by salt stress, suggesting that these genes may play important roles in R. trigyna's survival under high-salt environments. The method presented here successfully identified responsive genes from the massive amount of RNA-seq data. Thus, we suggest that DDRT-PCR could be employed to mine NGS data in a wide range of applications in transcriptomic studies. In addition, the genes identified in the present study are promising candidates for further elucidation of the salt tolerance mechanisms in R. trigyna.
机译:下一代测序(NGS)技术已用于从许多生物中生成大量测序数据。但是,使用这些遗传资源时,正确选择候选基因并防止从RNA-seq数据的数字基因表达(DGE)计算得出的假阳性结果至关重要。我们使用差异显示逆转录PCR(DDRT-PCR)与局部BLAST搜索相结合,从转录组测序数据中间接鉴定了18种盐胁迫诱导的Reaumuria trigyna转录本。与DGE结果高度一致,这些转录本的定量实时PCR表达模式显示出盐胁迫强烈上调,表明这些基因可能在高盐环境下的三角龙虾生存中发挥重要作用。此处介绍的方法已从大量的RNA-seq数据中成功鉴定出响应基因。因此,我们建议DDRT-PCR可用于转录组研究中广泛的应用中挖掘NGS数据。另外,在本研究中鉴定的基因是有希望的候选者,用于进一步阐明三角龙虾的耐盐性机制。

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