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Validation of reference genes for quantitative RT-PCR normalization in Suaeda aralocaspica an annual halophyte with heteromorphism and C4 pathway without Kranz anatomy

机译:一年生盐生植物具有异型性和C4途径而没有Kranz解剖的Suaeda aralocaspica中定量RT-PCR标准化参考基因的验证

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摘要

Reverse transcription quantitative real-time polymerase chain reaction (qRT-PCR) is a powerful analytical technique for the measurement of gene expression, which depends on the stability of the reference gene used for data normalization. Suaeda aralocaspica, an annual halophyte with heteromorphic seeds and possessing C4 photosynthesis pathway without Kranz anatomy, is an ideal plant species to identify stress tolerance-related genes and compare relative expression at transcriptional level. So far, no molecular information is available for this species. In the present study, six traditionally used reference genes were selected and their expression stability in two types of seeds of S. aralocaspica under different experimental conditions was evaluated. Three analytical programs, geNorm, NormFinder and BestKeeper, were used to assess and rank the stability of reference gene expression. Results revealed that although some reference genes may display different transcriptional profiles between the two types of seeds, β-TUB and GAPDH appeared to be the most suitable references under different developmental stages and tissues. GAPDH was the appropriate reference gene under different germination time points and salt stress conditions, and ACTIN was suitable for various abiotic stress treatments for the two types of seeds. For all the sample pools, β-TUB served as the most stable reference gene, whereas 18S rRNA and 28S rRNA performed poorly and presented as the least stable genes in our study. UBQ seemed to be unsuitable as internal control under different salt treatments. In addition, the expression of a photosynthesis-related gene (PPDK) of C4 pathway and a salt tolerance-related gene (SAT) of S. aralocaspica were used to validate the best performance reference genes. This is the first systematic comparison of reference gene selection for qRT-PCR work in S. aralocaspica and these data will facilitate further studies on gene expression in this species and other euhalophytes.
机译:逆转录实时定量聚合酶链反应(qRT-PCR)是一种强大的分析技术,可用于测量基因表达,这取决于用于数据标准化的参考基因的稳定性。 Suaeda aralocaspica是一年生盐生植物,具有异形种子,并具有无需Kranz解剖结构的C4光合作用途径,是一种理想的植物物种,可识别与胁迫耐受性相关的基因并在转录水平上比较相对表达。到目前为止,尚无该物种的分子信息。在本研究中,选择了六个传统使用的参考基因,并评估了它们在不同实验条件下在两种阿拉伯链霉菌种子中的表达稳定性。使用三个分析程序geNorm,NormFinder和BestKeeper评估参考基因表达的稳定性并对其进行排名。结果表明,尽管某些参考基因在两种类型的种子之间可能表现出不同的转录谱,但在不同的发育阶段和组织下,β-TUB和GAPDH似乎是最合适的参考。 GAPDH是在不同发芽时间点和盐胁迫条件下的适当参考基因,而ACTIN适用于两种类型种子的各种非生物胁迫处理。对于所有样本库,β-TUB充当最稳定的参考基因,而18S rRNA和28S rRNA表现不佳,在我们的研究中表现为最不稳定的基因。 UBQ似乎不适合作为在不同盐处理下的内部控制。此外,C4途径的光合作用相关基因(PPDK)和阿拉伯糖链霉菌的耐盐性相关基因(SAT)的表达被用来验证最佳性能参考基因。这是在阿拉伯糖链霉菌中进行qRT-PCR工作的参考基因选择的首次系统比较,这些数据将有助于对该物种和其他真核生物中基因表达的进一步研究。

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