首页> 外文期刊>Journal of Neuroscience Methods >The use of TaqMan RT-PCR assays for semiquantitative analysis of gene expression in CNS tissues and disease models.
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The use of TaqMan RT-PCR assays for semiquantitative analysis of gene expression in CNS tissues and disease models.

机译:使用TaqMan RT-PCR分析法对CNS组织和疾病模型中的基因表达进行半定量分析。

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TaqMan reverse transcription polymerase chain reaction (RT-PCR) is a recently developed technique which allows the measurement of an accumulating PCR product in real time. In the present study we have validated the use of TaqMan RT-PCR for mRNA localisation studies in human and rat tissues, and for the investigation of gene expression changes in CNS animal models. In human brain, D(2) receptor mRNA was enriched in caudate nucleus and putamen, whilst in rat brain, highest levels of D(2) receptor mRNA expression were observed in striatum and nucleus accumbens, consistent with the known distribution of this receptor in basal ganglia. In a rat model of permanent middle cerebral artery occlusion (pMCAO), endogenous interleukin-1 receptor antagonist (IL-1ra) mRNA was upregulated over 30-fold at 24 h post-lesion in both striatum and cortex ipsilateral to artery occlusion. Brain-derived neurotrophic factor (BDNF) mRNA was transiently upregulated 3.7-fold at 3 h, but not at 24 h or 3 days after induction of cortical spreading depression (CSD) in rats. Our observations in these two animal models using TaqMan RT-PCR were consistent with previous reports using other techniques. In conclusion, TaqMan RT-PCR assays provide a rapid and reliable method for semi-quantitative analysis of gene expression in the nervous system.
机译:TaqMan逆转录聚合酶链反应(RT-PCR)是一项最新开发的技术,可实时测量累积的PCR产物。在本研究中,我们已经验证了TaqMan RT-PCR在人类和大鼠组织中的mRNA定位研究以及CNS动物模型中基因表达变化的研究中的应用。在人脑中,D(2)受体mRNA富集在尾状核和壳状核中,而在大鼠脑中,纹状体和伏隔核中观察到最高水平的D(2)受体mRNA表达,与该受体在肝脏中的已知分布相一致。基底神经节。在大鼠大脑中动脉永久闭塞(pMCAO)的模型中,损伤后24 h,纹状体和大脑皮层同侧的内源性白介素1受体拮抗剂(IL-1ra)mRNA上调了30倍以上。在诱导皮层扩散抑制(CSD)后的3小时,但不是在24小时或3天,脑源性神经营养因子(BDNF)mRNA瞬时上调了3.7倍。我们使用TaqMan RT-PCR在这两种动物模型中的观察结果与先前使用其他技术的报道一致。总之,TaqMan RT-PCR分析提供了一种快速可靠的方法,用于神经系统基因表达的半定量分析。

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