用于全基因组表达研究的定量cDNA-AFLP分析

Quantitative cDNA-AFLP analysis for genome-wide expression studies.

作者信息

Breyne P, Dreesen R, Cannoot B, Rombaut D, Vandepoele K, Rombauts S, Vanderhaeghen R, Inzé D, Zabeau M

机构信息

Department of Plant Systems Biology, Flanders Interuniversity Institute for Biotechnology, Ghent University, K.L. Ledeganckstraat 35, Belgium.

出版信息

Mol Genet Genomics. 2003 May;269(2):173-9. doi: 10.1007/s00438-003-0830-6. Epub 2003 Mar 18.

DOI:10.1007/s00438-003-0830-6

PMID:12756529

Abstract

An improved cDNA-AFLP method for genome-wide expression analysis has been developed. We demonstrate that this method is an efficient tool for quantitative transcript profiling and a valid alternative to microarrays. Unique transcript tags, generated from reverse-transcribed messenger RNA by restriction enzymes, were screened through a series of selective PCR amplifications. Based on in silico analysis, an enzyme combination was chosen that ensures that at least 60% of all the mRNAs were represented by an informative sequence tag. The sensitivity and specificity of the method allows one to detect poorly expressed genes and distinguish between homologous sequences. Accurate gene expression profiles were determined by quantitative analysis of band intensities, and subtle differences in transcriptional activity were revealed. A detailed screen for cell cycle-modulated genes in tobacco demonstrates the usefulness of the technology for genome-wide expression analysis.

摘要

一种用于全基因组表达分析的改进型cDNA-AFLP方法已经开发出来。我们证明该方法是定量转录谱分析的有效工具，也是微阵列的有效替代方法。通过限制性酶从逆转录的信使RNA产生的独特转录标签，通过一系列选择性PCR扩增进行筛选。基于计算机分析，选择了一种酶组合，以确保所有mRNA中至少60%由信息序列标签代表。该方法的灵敏度和特异性使人们能够检测低表达基因并区分同源序列。通过对条带强度的定量分析确定了准确的基因表达谱，并揭示了转录活性的细微差异。对烟草中细胞周期调控基因的详细筛选证明了该技术在全基因组表达分析中的实用性。

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用于全基因组表达研究的定量cDNA-AFLP分析

Quantitative cDNA-AFLP analysis for genome-wide expression studies.

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