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首页> 外文期刊>Plant Science: An International Journal of Experimental Plant Biology >Screening of valid reference genes for real-time RT-PCR data normalization in Hevea brasiliensis and expression validation of a sucrose transporter gene HbSUT3.
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Screening of valid reference genes for real-time RT-PCR data normalization in Hevea brasiliensis and expression validation of a sucrose transporter gene HbSUT3.

机译:在巴西橡胶树中进行实时RT-PCR数据归一化的有效参考基因的筛选,以及蔗糖转运蛋白基因HbSUT3的表达验证。

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摘要

Real-time RT-PCR (RT-qPCR) is a sensitive and precise method of quantifying gene expression, however, suitable reference genes are required. Here, a systematic reference gene screening was performed by RT-qPCR on 22 candidate genes in Hevea brasiliensis. Two ubiquitin-protein ligases (UBC2a and UBC4) were the most stable when all samples were analyzed together. A mitosis protein (YLS8) and a eukaryotic translation initiation factor (eIF1Aa) were the most stable in response to tapping. UBC2b and UBC1 were the most stable among different genotypes. UBC2b and a DEAD box RNA helicase (RH2b) were the most stable across individual trees. YLS8 and RH8 were most stably expressed in hormone-treated samples. Expression of the candidate reference genes varied significantly across different tissues, and at least four genes (RH2b, RH8, UBC2a and eIF2) were needed for expression normalization. In addition, examination of relative expression of a sucrose transporter HbSUT3 in different RNA samples demonstrated the importance of additional reference genes to ensure accurate quantitative expression analysis. Overall, our work serves as a guide for selection of reference genes in RT-qPCR gene expression studies in H. brasiliensis.
机译:实时RT-PCR(RT-qPCR)是量化基因表达的灵敏且精确的方法,但是需要合适的参考基因。在此,通过RT-qPCR对巴西橡胶树中的22个候选基因进行了系统的参考基因筛选。当一起分析所有样品时,两种泛素蛋白连接酶( UBC2a 和 UBC4 )最稳定。有丝分裂蛋白( YLS8 )和真核翻译起始因子( eIF1Aa )对敲击响应最稳定。在不同基因型中, UBC2b 和 UBC1 最稳定。 UBC2b 和DEAD box RNA解旋酶( RH2b )在每棵树上最稳定。 YLS8 和 RH8 在激素处理过的样品中最稳定地表达。候选参考基因在不同组织中的表达差异很大,并且至少有四个基因( RH2b , RH8 , UBC2a 和 eIF2 < / i>)用于表达标准化。此外,检查蔗糖转运蛋白HbSUT3在不同RNA样品中的相对表达证明了其他参考基因对确保准确的定量表达分析的重要性。总体而言,我们的工作可作为在H进行RT-qPCR基因表达研究中选择参考基因的指南。巴西利亚

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