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基于大样本精神疾病尸检脑组织标本的 RT-qPCR 研究:内参基因与样本特征

RT-qPCR study on post-mortem brain samples from patients with major psychiatric disorders: reference genes and specimen characteristics.

机构信息

Hospital Universitari Psiquiàtric Institut Pere Mata, IISPV. Universitat Rovira i Virgili, C/ Sant Llorenç 21, 43201 Reus, Spain.

出版信息

J Psychiatr Res. 2011 Nov;45(11):1411-8. doi: 10.1016/j.jpsychires.2011.06.001. Epub 2011 Jun 24.

Abstract

BACKGROUND

Gene expression studies conducted in post-mortem human brain samples have the potential to identify relevant genes implicated in psychiatric disorders. Although reverse transcription quantitative real-time PCR (RT-qPCR) has emerged as the method of choice for specific gene expression studies, it requires the use of stable reference genes, and it is necessary to control for pre- and post-mortem factors to obtain reliable data.

OBJECTIVE

The aim of this study was to identify suitable reference genes and specimen characteristics that can be taken into account when comparing mRNA expression data between post-mortem brain specimens from psychiatric patients and controls.

METHOD

We used a selection of suitably matched occipital cortex specimens from subjects in each of the following groups: schizophrenia (N = 15), bipolar disorder (N = 13), major depressive disorder (N = 15), and control (N = 15). Quantitative and qualitative RNA analyses were performed prior to RT-qPCR and gene expression stability was evaluated with geNorm and NormFinder.

RESULTS

We identified GAPDH, RPS17, RPL30, RPLP0, and TFRC as potential reference genes from a sample plate containing 32 candidates commonly used as reference genes. Further analyses of these 5 genes highlighted that 1) they are suitable reference genes for RT-qPCR studies in these post-mortem brain samples from psychiatric patients, and 2) the RNA quality index is highly correlated with gene expression values (r = -0.681, p < 0.0001).

CONCLUSIONS

In addition to controlling for pre- and post-mortem factors and selecting stable reference genes for normalization, sample sets should be matched with regard to RNA quality.

摘要

背景

在死后的人脑样本中进行的基因表达研究有潜力鉴定出与精神疾病相关的基因。虽然逆转录实时定量 PCR (RT-qPCR)已成为特定基因表达研究的首选方法,但它需要使用稳定的参照基因,并需要控制生前和死后的因素,以获得可靠的数据。

目的

本研究旨在鉴定合适的参照基因和样本特征,在比较精神病患者和对照死后脑样本的 mRNA 表达数据时,可以考虑这些因素。

方法

我们使用了来自以下各组的适当匹配的枕叶皮质样本:精神分裂症 (N=15)、双相情感障碍 (N=13)、重性抑郁障碍 (N=15)和对照 (N=15)。在进行 RT-qPCR 之前进行了定量和定性 RNA 分析,并使用 geNorm 和 NormFinder 评估了基因表达稳定性。

结果

我们从一个包含 32 个常用作参照基因的候选基因的样本板中确定了 GAPDH、RPS17、RPL30、RPLP0 和 TFRC 作为潜在的参照基因。对这 5 个基因的进一步分析表明,1)它们是这些来自精神病患者死后脑样本的 RT-qPCR 研究的合适参照基因,2)RNA 质量指数与基因表达值高度相关 (r=-0.681,p<0.0001)。

结论

除了控制生前和死后的因素以及选择稳定的参照基因进行归一化外,样本集还应在 RNA 质量方面进行匹配。

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