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Identification of condition-specific reference genes from microarray data for locusts exposed to hypobaric hypoxia

机译:从微阵列数据中鉴定低氧缺氧蝗虫的条件特异性参考基因

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Real-time quantitative polymerase chain reaction (qPCR) is a routine and robust approach for measuring gene expression. The stability of reference genes in qPCR is crucial for the accurate quantification of gene expression. To provide reliable reference genes for studying the transcriptional responses of locust muscles to hypobaric hypoxia, we first examined the gene expression stability of the frequently used housekeeping genes 18S, GAPDH, and @b-actin. However, the expression of these three housekeeping genes was influenced by hypobaric hypoxia. Consequently, we identified five novel candidate reference genes from the locust microarray data. The gene expression stability of the five candidates, together with the three classical housekeeping genes, were evaluated using two distinct algorithms implemented in geNorm and NormFinder. GeNorm identified Ach (acetyl-CoA hydrolase) and Pgp (phosphoglycolate phosphatase-like) as the most stable genes and NormFinder further distinguished Ach as the most stable one. The validity of Ach as a reference gene was confirmed through comparison with 18S. This study exemplifies the necessity of validating reference genes before their application and the feasibility of identifying condition-specific reference genes from large-scale gene expression data.
机译:实时定量聚合酶链反应(qPCR)是测量基因表达的常规且可靠的方法。 qPCR中参考基因的稳定性对于基因表达的准确定量至关重要。为了提供可靠的参考基因来研究蝗虫肌肉对低压缺氧的转录反应,我们首先检查了常用的管家基因18S,GAPDH和@ b-actin的基因表达稳定性。但是,这三个管家基因的表达受到低压缺氧的影响。因此,我们从蝗虫微阵列数据中鉴定出五个新颖的候选参考基因。使用在geNorm和NormFinder中实现的两种不同算法,评估了五个候选基因以及三个经典管家基因的基因表达稳定性。 GeNorm将Ach(乙酰辅酶A水解酶)和Pgp(磷酸甘氨酸磷酸酯酶样)鉴定为最稳定的基因,而NormFinder进一步将Ach鉴定为最稳定的基因。通过与18S的比较,确认了Ach作为参考基因的有效性。这项研究例证了在应用参考基因​​之前对其进行验证的必要性,以及从大规模基因表达数据中鉴定条件特异性参考基因的可行性。

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