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在红霉素应激条件下生长的头状葡萄球菌中用于基因表达研究的合适内参基因的筛选。

Selection of suitable reference genes for gene expression studies in Staphylococcus capitis during growth under erythromycin stress.

作者信息

Cui Bintao, Smooker Peter M, Rouch Duncan A, Deighton Margaret A

机构信息

School of Applied Sciences, RMIT University, Plenty Road, Bundoora, VIC, 3083, Australia.

出版信息

Mol Genet Genomics. 2016 Aug;291(4):1795-811. doi: 10.1007/s00438-016-1197-9. Epub 2016 Mar 21.

Abstract

Accurate and reproducible measurement of gene transcription requires appropriate reference genes, which are stably expressed under different experimental conditions to provide normalization. Staphylococcus capitis is a human pathogen that produces biofilm under stress, such as imposed by antimicrobial agents. In this study, a set of five commonly used staphylococcal reference genes (gyrB, sodA, recA, tuf and rpoB) were systematically evaluated in two clinical isolates of Staphylococcus capitis (S. capitis subspecies urealyticus and capitis, respectively) under erythromycin stress in mid-log and stationary phases. Two public software programs (geNorm and NormFinder) and two manual calculation methods, reference residue normalization (RRN) and relative quantitative (RQ), were applied. The potential reference genes selected by the four algorithms were further validated by comparing the expression of a well-studied biofilm gene (icaA) with phenotypic biofilm formation in S. capitis under four different experimental conditions. The four methods differed considerably in their ability to predict the most suitable reference gene or gene combination for comparing icaA expression under different conditions. Under the conditions used here, the RQ method provided better selection of reference genes than the other three algorithms; however, this finding needs to be confirmed with a larger number of isolates. This study reinforces the need to assess the stability of reference genes for analysis of target gene expression under different conditions and the use of more than one algorithm in such studies. Although this work was conducted using a specific human pathogen, it emphasizes the importance of selecting suitable reference genes for accurate normalization of gene expression more generally.

摘要

基因转录的准确且可重复测量需要合适的内参基因,这些基因在不同实验条件下稳定表达以提供标准化。头状葡萄球菌是一种人类病原体,在诸如抗菌剂施加的压力等条件下会产生生物膜。在本研究中,对一组五个常用的葡萄球菌内参基因(gyrB、sodA、recA、tuf和rpoB)在处于对数中期和稳定期的红霉素压力下,对头状葡萄球菌的两个临床分离株(分别为解脲脲原体亚种头状葡萄球菌和头状葡萄球菌)进行了系统评估。应用了两个公共软件程序(geNorm和NormFinder)以及两种手动计算方法,即参考残基归一化(RRN)和相对定量(RQ)。通过比较一个经过充分研究的生物膜基因(icaA)的表达与头状葡萄球菌在四种不同实验条件下的表型生物膜形成,对四种算法选择的潜在内参基因进行了进一步验证。这四种方法在预测用于比较不同条件下icaA表达的最合适内参基因或基因组合的能力上有很大差异。在此处使用的条件下,RQ方法比其他三种算法能更好地选择内参基因;然而,这一发现需要用更多的分离株来证实。本研究强化了在分析不同条件下靶基因表达时评估内参基因稳定性以及在此类研究中使用不止一种算法的必要性。尽管这项工作是使用一种特定的人类病原体进行的,但它更普遍地强调了选择合适的内参基因以准确归一化基因表达的重要性。

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