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监测基因表达:定量实时逆转录聚合酶链反应

Monitoring gene expression: quantitative real-time rt-PCR.

作者信息

Wagner Elke M

机构信息

Plasma Analytics/Development and Optimization, Baxter AG, Wien, Austria.

出版信息

Methods Mol Biol. 2013;1027:19-45. doi: 10.1007/978-1-60327-369-5_2.

DOI:10.1007/978-1-60327-369-5_2
PMID:23912981
Abstract

Two-step quantitative real-time RT-PCR (RT-qPCR), also known as real-time RT-PCR, kinetic RT-PCR, or quantitative fluorescent RT-PCR, has become the method of choice for gene expression analysis during the last few years. It is a fast and convenient PCR method that combines traditional RT-PCR with the phenomenon of fluorescence resonance energy transfer (FRET) using fluorogenic primers. The detection of changes in fluorescence intensity during the reaction enables the user to follow the PCR reaction in real time.RT-qPCR comprises several steps: (1) RNA is isolated from target tissue/cells; (2) mRNA is reverse-transcribed to cDNA; (3) modified gene-specific PCR primers are used to amplify a segment of the cDNA of interest, following the reaction in real time; and (4) the initial concentration of the selected transcript in a specific tissue or cell type is calculated from the exponential phase of the reaction. Relative quantification or absolute quantification compared to standards that are run in parallel can be performed.This chapter describes the entire procedure from isolation of total RNA from liver and fatty tissues/cells to the use of RT-qPCR to study gene expression in these tissues. We perform relative quantification of transcripts to calculate the fold-difference of a certain mRNA level between different samples. In addition, tips for choosing primers and performing analyses are provided to help the beginner in understanding the technique.

摘要

两步法定量实时逆转录聚合酶链反应(RT-qPCR),也称为实时RT-PCR、动力学RT-PCR或定量荧光RT-PCR,在过去几年中已成为基因表达分析的首选方法。它是一种快速便捷的PCR方法,将传统的RT-PCR与使用荧光引物的荧光共振能量转移(FRET)现象相结合。反应过程中荧光强度变化的检测使使用者能够实时跟踪PCR反应。RT-qPCR包括几个步骤:(1)从靶组织/细胞中分离RNA;(2)将mRNA逆转录为cDNA;(3)使用经过修饰的基因特异性PCR引物扩增感兴趣的cDNA片段,同时实时跟踪反应;(4)根据反应的指数期计算特定组织或细胞类型中所选转录本的初始浓度。可以与平行运行的标准品进行相对定量或绝对定量。本章描述了从肝脏和脂肪组织/细胞中分离总RNA到使用RT-qPCR研究这些组织中基因表达的整个过程。我们对转录本进行相对定量,以计算不同样品之间特定mRNA水平的倍数差异。此外,还提供了选择引物和进行分析的提示,以帮助初学者理解该技术。

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