An optimized RNA amplification method for prokaryotic expression profiling analysis

被引:0
|
作者
Feng-Lin Cao
Han-Hua Liu
Ya-Hui Wang
Yu Liu
Xiao-Yu Zhang
Jian-Qing Zhao
Yi-Min Sun
Jin Zhou
Liang Zhang
机构
[1] The First Clinical College of Harbin Medical University,The Institute of Hematology and Oncology of Heilongjiang Province
[2] National Engineering Research Center for Beijing Biochip Technology,The Cell Transplantation Key Laboratory of Health Ministry of China
[3] The First Clinical College of Harbin Medical University,undefined
来源
Applied Microbiology and Biotechnology | 2010年 / 87卷
关键词
Microarray analysis; Prokaryotic expression; RNA amplification; Target preparation method;
D O I
暂无
中图分类号
学科分类号
摘要
DNA microarray technology has been extensively used for gene expression analysis of both eukaryotic and prokaryotic organisms. For eukaryotic gene expression profiling, the poly(A)-based reverse transcription of messenger RNA (mRNA) followed by T7 RNA polymerase-based in vitro transcription is generally required to produce enough RNA targets for hybridization with the microarray chips. However, the same method cannot be directly applied to prokaryotic mRNAs due to the lack of poly(A) sequences at the 3′ ends. Conventional methods usually require large amounts of starting RNAs and lead to high background noise. Recently developed amplification methods enable smaller amounts of prokaryotic RNA to be used from samples with species-specific primers, oligo(dT) primers, or random primers. In this study, three target preparation methods, including the direct labeling, polyadenylation-involved oligo-dT priming, and random priming amplification (respectively referred to as DL, PAOD, and RPA hereafter) were evaluated through expression profiling of a heat shock model of Escherichia coli. The PAOD method was found to be more sensitive and more specific in differential gene expression measurements than either DL and RPA, even when the E. coli RNA was only a small proportion of the simulated eukaryotic host RNA. The results suggest that PAOD is the preferred target preparation method for prokaryotic transcriptome.
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页码:343 / 352
页数:9
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