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Selection of reliable reference genes for the normalisation of gene expression levels following time course LPS stimulation of murine bone marrow derived macrophages

机译:选择可靠的参考基因以使鼠骨髓来源的巨噬细胞经时程LPS刺激后的基因表达水平正常化

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摘要

BackgroundMacrophages are key players in the initiation, perpetuation and regulation of both innate and adaptive immune responses. They largely perform these roles through modulation of the expression of genes, especially those encoding cytokines. Murine bone marrow derived macrophages (BMDMs) are commonly used as a model macrophage population for the study of immune responses to pro-inflammatory stimuli, notably lipopolysaccharide (LPS), which may be pertinent to the human situation. Evaluation of the temporal responses of LPS stimulated macrophages is widely conducted via the measurement of gene expression levels by RT-qPCR. While providing a robust and sensitive measure of gene expression levels, RT-qPCR relies on the normalisation of gene expression data to a stably expressed reference gene. Generally, a normalisation gene(s) is selected from a list of “traditional” reference genes without validation of expression stability under the specific experimental conditions of the study. In the absence of such validation, and given that many studies use only a single reference gene, the reliability of data is questionable.
机译:背景巨噬细胞是先天性和适应性免疫反应的起始,永存和调节的关键参与者。它们主要通过调节基因的表达来发挥这些作用,尤其是编码细胞因子的基因。小鼠骨髓衍生的巨噬细胞(BMDM)通常用作模型巨噬细胞群体,用于研究对促炎性刺激的免疫反应,尤其是脂多糖(LPS),这可能与人类情况有关。 LPS刺激的巨噬细胞的时间响应的评估广泛地通过RT-qPCR测量基因表达水平来进行。 RT-qPCR在提供可靠且敏感的基因表达水平衡量指标的同时,还依赖于将基因表达数据标准化为稳定表达的参考基因的方法。通常,归一化基因是从“传统”参考基因列表中选择的,而没有在研究的特定实验条件下验证表达稳定性。在没有这种验证的情况下,并且鉴于许多研究仅使用单个参考基因,因此数据的可靠性值得怀疑。

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