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Reference genes selection for Calotropis procera under different salt stress conditions

机译:盐胁迫条件下中华螯虾的参考基因选择。

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摘要

Calotropis procera is a perennial Asian shrub with significant adaptation to adverse climate conditions and poor soils. Given its increased salt and drought stress tolerance, C. procera stands out as a powerful candidate to provide alternative genetic resources for biotechnological approaches. The qPCR (real-time quantitative polymerase chain reaction), widely recognized among the most accurate methods for quantifying gene expression, demands suitable reference genes (RGs) to avoid over- or underestimations of the relative expression and incorrect interpretation. This study aimed at evaluating the stability of ten RGs for normalization of gene expression of root and leaf of C. procera under different salt stress conditions and different collection times. The selected RGs were used on expression analysis of three target genes. Three independent experiments were carried out in greenhouse with young plants: i) Leaf100 = leaf samples collected 30 min, 2 h, 8 h and 45 days after NaCl-stress (100 mM NaCl); ii) Root50 and iii) Root200 = root samples collected 30 min, 2 h, 8 h and 1day after NaCl-stress (50 and 200 mM NaCl, respectively). Stability rank among the three algorithms used showed high agreement for the four most stable RGs. The four most stable RGs showed high congruence among all combination of collection time, for each software studied, with minor disagreements. CYP23 was the best RG (rank of top four) for all experimental conditions (Leaf100, Root50, and Root200). Using appropriated RGs, we validated the relative expression level of three differentially expressed target genes (NAC78, CNBL4, and ND1) in Leaf100 and Root200 samples. This study provides the first selection of stable reference genes for C. procera under salinity. Our results emphasize the need for caution when evaluating the stability RGs under different amplitude of variable factors.
机译:Calotropis procera是一种多年生亚洲灌木,对不利的气候条件和土壤贫瘠具有明显的适应性。鉴于其对盐和干旱胁迫的耐受性增强,proc。procera成为为生物技术方法提供替代遗传资源的有力候选者。 qPCR(实时定量聚合酶链反应)是最准确的定量基因表达方法之一,它需要合适的参考基因(RGs)来避免相对表达的过高或过低以及错误的解释。本研究旨在评估在不同盐胁迫条件和不同收集时间下,十倍体RGs稳定过​​程的根和叶基因表达的稳定性。选择的RG用于三个靶基因的表达分析。在有幼植物的温室中进行了三个独立的实验:i)叶100 = NaCl胁迫(100 mM NaCl)后30分钟,2小时,8小时和45天收集的叶片样品; ii)根50和iii)根200 = NaCl胁迫后30分钟,2小时,8小时和1天(分别为50和200 mM NaCl)收集的根样品。所使用的三种算法中的稳定性等级显示出对于四个最稳定的RG的高度一致性。对于所研究的每种软件,四个最稳定的RG在收集时间的所有组合中均显示出较高的一致性,但有较小的分歧。 CYP23是所有实验条件(Leaf100,Root50和Root200)的最佳RG(前四名)。使用适当的RG,我们验证了Leaf100和Root200样品中三个差异表达的靶基因(NAC78,CNBL4和ND1)的相对表达水平。这项研究为盐度下的proc。procera提供了稳定的参考基因的首选。我们的结果强调在评估可变因素不同幅度下的稳定性RG时需要谨慎。

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