共 46 条
Evaluation of methods for amplification of picogram amounts of total RNA for whole genome expression profiling
被引:46
作者:

Clement-Ziza, Mathieu
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机构:
Univ Paris 05, INSERM U781, Fac Med, Hop Necker Enfants Malad, F-75015 Paris, France Inst Curie, Dept Transfert, F-75248 Paris 05, France

Gentien, David
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Inst Curie, Dept Transfert, F-75248 Paris 05, France Inst Curie, Dept Transfert, F-75248 Paris 05, France

Lyonnet, Stanislas
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机构:
Univ Paris 05, INSERM U781, Fac Med, Hop Necker Enfants Malad, F-75015 Paris, France Inst Curie, Dept Transfert, F-75248 Paris 05, France

Thiery, Jean-Paul
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机构:
Inst Curie, Dept Transfert, F-75248 Paris 05, France
IMCB Proteos, Singapore 138673, Singapore Inst Curie, Dept Transfert, F-75248 Paris 05, France

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Decraene, Charles
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机构:
Inst Curie, Dept Transfert, F-75248 Paris 05, France
Inst Curie, Ctr Rech, F-75248 Paris 05, France
CNRS, UMR144, F-75248 Paris 05, France Inst Curie, Dept Transfert, F-75248 Paris 05, France
机构:
[1] Inst Curie, Dept Transfert, F-75248 Paris 05, France
[2] Univ Paris 05, INSERM U781, Fac Med, Hop Necker Enfants Malad, F-75015 Paris, France
[3] IMCB Proteos, Singapore 138673, Singapore
[4] Inst Curie, Ctr Rech, F-75248 Paris 05, France
[5] CNRS, UMR144, F-75248 Paris 05, France
来源:
关键词:
LASER CAPTURE MICRODISSECTION;
GENE-EXPRESSION;
MICROARRAY ANALYSIS;
LINEAR AMPLIFICATION;
OLIGONUCLEOTIDE MICROARRAYS;
NANOGRAM AMOUNTS;
SMALL SAMPLES;
CELLS;
CDNA;
HYBRIDIZATION;
D O I:
10.1186/1471-2164-10-246
中图分类号:
Q81 [生物工程学(生物技术)];
Q93 [微生物学];
学科分类号:
071005 ;
0836 ;
090102 ;
100705 ;
摘要:
Background: For more than a decade, microarrays have been a powerful and widely used tool to explore the transcriptome of biological systems. However, the amount of biological material from cell sorting or laser capture microdissection is much too small to perform microarray studies. To address this issue, RNA amplification methods have been developed to generate sufficient targets from picogram amounts of total RNA to perform microarray hybridisation. Results: In this study, four commercial protocols for amplification of picograms amounts of input RNA for microarray expression profiling were evaluated and compared. The quantitative and qualitative performances of the methods were assessed. Microarrays were hybridised with the amplified targets and the amplification protocols were compared with respect to the quality of expression profiles, reproducibility within a concentration range of input RNA, and sensitivity. The results demonstrate significant differences between these four methods. Conclusion: In our hands, the WT-Ovation pico system proposed by Nugen appears to be the most suitable for RNA amplification. This comparative study will be useful to scientists needing to choose an amplification method to carry out microarray experiments involving samples comprising only a few cells and generating picogram amounts of RNA.
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