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确定不同组织和小鼠品系中 circadian 研究的参考基因。

Determination of reference genes for circadian studies in different tissues and mouse strains.

机构信息

Faculty of Medicine, Center for Functional Genomics and Bio-Chips, Institute of Biochemistry, University of Ljubljana, Zaloska 4, SI-1000 Ljubljana, Slovenia.

出版信息

BMC Mol Biol. 2010 Aug 16;11:60. doi: 10.1186/1471-2199-11-60.

Abstract

BACKGROUND

Circadian rhythms have a profound effect on human health. Their disruption can lead to serious pathologies, such as cancer and obesity. Gene expression studies in these pathologies are often studied in different mouse strains by quantitative real time polymerase chain reaction (qPCR). Selection of reference genes is a crucial step of qPCR experiments. Recent studies show that reference gene stability can vary between species and tissues, but none has taken circadian experiments into consideration.

RESULTS

In the present study the expression of ten candidate reference genes (Actb, Eif2a, Gapdh, Hmbs, Hprt1, Ppib, Rn18s, Rplp0, Tbcc and Utp6c) was measured in 131 liver and 97 adrenal gland samples taken from three mouse strains (C57BL/6JOlaHsd, 129Pas plus C57BL/6J and Crem KO on 129Pas plus C57BL/6J background) every 4 h in a 24 h period. Expression stability was evaluated by geNorm and NormFinder programs. Differences in ranking of the most stable reference genes were observed both between individual mouse strains as well as between tissues within each mouse strain. We show that selection of reference gene (Actb) that is often used for analyses in individual mouse strains leads to errors if used for normalization when different mouse strains are compared. We identified alternative reference genes that are stable in these comparisons.

CONCLUSIONS

Genetic background and circadian time influence the expression stability of reference genes. Differences between mouse strains and tissues should be taken into consideration to avoid false interpretations. We show that the use of a single reference gene can lead to false biological conclusions. This manuscript provides a useful reference point for researchers that search for stable reference genes in the field of circadian biology.

摘要

背景

昼夜节律对人类健康有深远的影响。其紊乱可导致严重的病变,如癌症和肥胖。这些病变的基因表达研究通常通过定量实时聚合酶链反应(qPCR)在不同的小鼠品系中进行。参考基因的选择是 qPCR 实验的关键步骤。最近的研究表明,参考基因的稳定性可能因物种和组织而异,但尚未考虑昼夜节律实验。

结果

在本研究中,我们在三种小鼠品系(C57BL/6JOlaHsd、129Pas plus C57BL/6J 和 Crem KO on 129Pas plus C57BL/6J 背景)的 131 个肝脏和 97 个肾上腺样本中,每 4 小时测量了 10 个候选参考基因(Actb、Eif2a、Gapdh、Hmbs、Hprt1、Ppib、Rn18s、Rplp0、Tbcc 和 Utp6c)的表达。使用 geNorm 和 NormFinder 程序评估表达稳定性。在个体小鼠品系之间以及每个小鼠品系的组织内,观察到最稳定的参考基因的排名差异。我们表明,在比较不同的小鼠品系时,如果使用常用于个体小鼠品系分析的参考基因(Actb)进行归一化,会导致错误。我们确定了在这些比较中稳定的替代参考基因。

结论

遗传背景和昼夜节律时间会影响参考基因的表达稳定性。应考虑小鼠品系和组织之间的差异,以避免错误的解释。我们表明,使用单个参考基因可能会导致错误的生物学结论。本文为昼夜生物学领域寻找稳定参考基因的研究人员提供了有用的参考点。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f85e/2928770/b0bee1a3cdc4/1471-2199-11-60-1.jpg

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