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利用激光捕获显微切割技术和微阵列对单只动物的各个下丘脑核团进行基因表达谱分析。

Gene expression profiling of individual hypothalamic nuclei from single animals using laser capture microdissection and microarrays.

作者信息

Paulsen Sarah Juel, Larsen Leif Kongskov, Jelsing Jacob, Janssen Uwe, Gerstmayer Bernhard, Vrang Niels

机构信息

Rheoscience A/S, Glerupvej 1, DK-2610 Rødovre, Denmark; University of Southern Denmark, BMB, Campusvej 55, DK-5230 Odense M, Denmark.

出版信息

J Neurosci Methods. 2009 Feb 15;177(1):87-93. doi: 10.1016/j.jneumeth.2008.09.024. Epub 2008 Oct 8.

DOI:10.1016/j.jneumeth.2008.09.024
PMID:18955080
Abstract

In order to identify novel genes involved in appetite and body weight regulation we have developed a microarray based method suitable for detecting small changes in gene expression in discrete groups of hypothalamic neurons. The method is based on a combination of stereological sampling, laser capture microdissection (LCM), PCR based amplification (SuperAmp), and one-color cDNA microarray analysis. To validate the method we assessed and compared fasting induced changes in mRNA levels of Neuropeptide Y (NPY) and proopiomelanocortin (POMC) in the hypothalamic arcuate nucleus (ARC) of diet-induced obese rats using cDNA microarrays, quantitative PCR and in situ hybridization. All methods revealed statistically significant fasting-induced changes in NPY and POMC expression. An additional 3480 differentially expressed probes (fold change >1.22, t-test p=0.05) were identified in the microarray analysis. Our findings demonstrate a consistent gene expression pattern across three different gene expression detection methods and strongly suggest that LCM coupled microarray analysis combined with SuperAmp can be used as a semi-quantitative mRNA profiling tool. Importantly, the sensitivity of the method greatly improves the usefulness of the microarray technology for gene expression profiling in non-homogeneous tissues such as the brain.

摘要

为了鉴定参与食欲和体重调节的新基因,我们开发了一种基于微阵列的方法,该方法适用于检测下丘脑离散神经元群中基因表达的微小变化。该方法基于体视学采样、激光捕获显微切割(LCM)、基于PCR的扩增(SuperAmp)和单色cDNA微阵列分析的组合。为了验证该方法,我们使用cDNA微阵列、定量PCR和原位杂交评估并比较了饮食诱导肥胖大鼠下丘脑弓状核(ARC)中禁食诱导的神经肽Y(NPY)和阿黑皮素原(POMC)mRNA水平的变化。所有方法均显示禁食诱导的NPY和POMC表达变化具有统计学意义。在微阵列分析中还鉴定出另外3480个差异表达探针(倍数变化>1.22,t检验p = 0.05)。我们的研究结果表明,三种不同基因表达检测方法具有一致的基因表达模式,并强烈表明LCM耦合微阵列分析与SuperAmp相结合可作为一种半定量mRNA分析工具。重要的是,该方法的灵敏度大大提高了微阵列技术在非均质组织(如大脑)中进行基因表达谱分析的实用性。

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