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Normalisation genes for expression analyses in the brown alga model Ectocarpus siliculosus

机译:用于褐藻模型Ectocarpus siliculosus表达分析的归一化基因

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Background Brown algae are plant multi-cellular organisms occupying most of the world coasts and are essential actors in the constitution of ecological niches at the shoreline. Ectocarpus siliculosus is an emerging model for brown algal research. Its genome has been sequenced, and several tools are being developed to perform analyses at different levels of cell organization, including transcriptomic expression analyses. Several topics, including physiological responses to osmotic stress and to exposure to contaminants and solvents are being studied in order to better understand the adaptive capacity of brown algae to pollution and environmental changes. A series of genes that can be used to normalise expression analyses is required for these studies. Results We monitored the expression of 13 genes under 21 different culture conditions. These included genes encoding proteins and factors involved in protein translation (ribosomal protein 26S, EF1alpha, IF2A, IF4E) and protein degradation (ubiquitin, ubiquitin conjugating enzyme) or folding (cyclophilin), and proteins involved in both the structure of the cytoskeleton (tubulin alpha, actin, actin-related proteins) and its trafficking function (dynein), as well as a protein implicated in carbon metabolism (glucose 6-phosphate dehydrogenase). The stability of their expression level was assessed using the Ct range, and by applying both the geNorm and the Normfinder principles of calculation. Conclusion Comparisons of the data obtained with the three methods of calculation indicated that EF1alpha (EF1a) was the best reference gene for normalisation. The normalisation factor should be calculated with at least two genes, alpha tubulin, ubiquitin-conjugating enzyme or actin-related proteins being good partners of EF1a. Our results exclude actin as a good normalisation gene, and, in this, are in agreement with previous studies in other organisms.
机译:背景技术褐藻是占据世界大部分沿海地区的植物多细胞生物,并且是构成海岸线生态位的重要因素。 Ectocarpus siliculosus是棕色藻类研究的新兴模型。已经对其基因组进行了测序,并且正在开发几种工具来在细胞组织的不同水平上进行分析,包括转录组表达分析。为了更好地了解褐藻对污染和环境变化的适应能力,正在研究几个主题,包括对渗透压的生理反应以及对污染物和溶剂的暴露。这些研究需要一系列可用于标准化表达分析的基因。结果我们监测了21种不同培养条件下13个基因的表达。这些基因包括编码蛋白质和参与蛋白质翻译的因子(核糖体蛋白26S,EF1alpha,IF2A,IF4E)和蛋白质降解(泛素,泛素结合酶)或折叠(亲环素)的基因,以及参与细胞骨架结构(微管蛋白)的蛋白质α,肌动蛋白,肌动蛋白相关蛋白)及其运输功能(达因)以及涉及碳代谢的蛋白(6-磷酸葡萄糖脱氢酶)。使用Ct范围并通过应用geNorm和Normfinder计算原理来评估其表达水平的稳定性。结论通过三种计算方法获得的数据比较表明,EF1alpha(EF1a)是标准化的最佳参考基因。归一化因子应使用至少两个基因(EF1a的良好伴侣)来计算,即α微管蛋白,泛素结合酶或肌动蛋白相关蛋白。我们的结果排除了肌动蛋白作为良好的归一化基因,并且在此方面与先前在其他生物中的研究一致。

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