Literature DB >> 15613496

Microarray-based comparison of three amplification methods for nanogram amounts of total RNA.

Ruchira Singh1, Rajanikanth J Maganti, Sairam V Jabba, Martin Wang, Glenn Deng, Joe Don Heath, Nurith Kurn, Philine Wangemann.   

Abstract

Gene expression profiling using microarrays requires microgram amounts of RNA, which limits its direct application for the study of nanogram RNA samples obtained using microdissection, laser capture microscopy, or needle biopsy. A novel system based on Ribo-SPIA technology (RS, Ovation-Biotin amplification and labeling system) was recently introduced. The utility of the RS system, an optimized prototype system for picogram RNA samples (pRS), and two T7-based systems involving one or two rounds of amplification (One RA, Standard Protocol, or Two RA, Small Sample Prototcol, version II) were evaluated in the present study. Mouse kidney (MK) and mouse universal reference (MUR) RNA samples, 0.3 ng to 10 mug, were analyzed using high-density Affymetrix Mouse Genome 430 2.0 GeneChip arrays. Call concordance between replicates, correlations of signal intensity, signal intensity ratios, and minimal fold increase necessary for significance were determined. All systems amplified partially overlapping sets of genes with similar signal intensity correlations. pRS amplified the highest number of genes from 10-ng RNA samples. We detected 24 of 26 genes verified by RT-PCR in samples prepared using pRS. Two RA yielded somewhat higher call concordances than did RS and pRS (91.8% vs. 89.3% and 88.1%, respectively). Although all target preparation methods were suitable, pRS amplified the highest number of targets and was found to be suitable for amplification of as little as 0.3 ng of total RNA. In addition, RS and pRS were faster and simpler to use than the T7-based methods and resulted in the generation of cDNA, which is more stable than cRNA.

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Year:  2004        PMID: 15613496      PMCID: PMC2020524          DOI: 10.1152/ajpcell.00258.2004

Source DB:  PubMed          Journal:  Am J Physiol Cell Physiol        ISSN: 0363-6143            Impact factor:   4.249


  22 in total

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Authors:  L R Baugh; A A Hill; E L Brown; C P Hunter
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3.  Optimized T7 amplification system for microarray analysis.

Authors:  C Pabón; Z Modrusan; M V Ruvolo; I M Coleman; S Daniel; H Yue; L J Arnold
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4.  A PCR-based amplification method retaining the quantitative difference between two complex genomes.

Authors:  G Mike Makrigiorgos; Subrata Chakrabarti; Yuzhi Zhang; Manjit Kaur; Brendan D Price
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5.  Advantages of mRNA amplification for microarray analysis.

Authors:  A L Feldman; N G Costouros; E Wang; M Qian; F M Marincola; H R Alexander; S K Libutti
Journal:  Biotechniques       Date:  2002-10       Impact factor: 1.993

6.  Representation is faithfully preserved in global cDNA amplified exponentially from sub-picogram quantities of mRNA.

Authors:  Norman N Iscove; Mary Barbara; Marie Gu; Meredith Gibson; Carolyn Modi; Neil Winegarden
Journal:  Nat Biotechnol       Date:  2002-08-12       Impact factor: 54.908

7.  High-accuracy amplification of nanogram total RNA amounts for gene profiling.

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8.  Amplified RNA synthesized from limited quantities of heterogeneous cDNA.

Authors:  R N Van Gelder; M E von Zastrow; A Yool; W C Dement; J D Barchas; J H Eberwine
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10.  Prokaryotic RNA preparation methods useful for high density array analysis: comparison of two approaches.

Authors:  C Rosenow; R M Saxena; M Durst; T R Gingeras
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  31 in total

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4.  Comparison of RNA amplification techniques meeting the demands for the expression profiling of clinical cancer samples.

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Review 7.  Review of the literature examining the correlation among DNA microarray technologies.

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8.  Developmental delays consistent with cochlear hypothyroidism contribute to failure to develop hearing in mice lacking Slc26a4/pendrin expression.

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9.  Evaluation of methods for amplification of picogram amounts of total RNA for whole genome expression profiling.

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10.  Gene expression profiling of whole blood: comparison of target preparation methods for accurate and reproducible microarray analysis.

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