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      • Record: found
      • Abstract: found
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      Multiplexed measurements of gene signatures in different analytes using the Nanostring nCounter™ Assay System

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          Abstract

          Background

          We assessed NanoString's nCounter™ Analysis System for its ability to quantify gene expression of forty-eight genes in a single reaction with 100 ng of total RNA or an equivalent amount of tissue lysate. In the nCounter™ System, multiplexed gene expression target levels are directly detected, without enzymatic reactions, via two sequence-specific probes. The individual mRNA is captured with one mRNA target sequence-specific capture probe that is used in a post-hybridization affinity purification procedure. The second mRNA target specific-sequence and fluorescent-labeled colored coded probe is then used in the detection with the 3-component complex separated on a surface via an applied electric field followed by imaging. We evaluated reproducibility, accuracy, concordance with quantitative RT-PCR, linearity, dynamic range, and the ability of the system to assay different inputs (matched samples of total RNA from Flash Frozen (FF) and Formalin Fixed Paraffin Embedded Tissues (FFPET), and crude tissue lysates (CTL)).

          Findings

          The nCounter™ Analysis System provided data equivalent to that produced by Taqman ®-based assays for genes expressed within the ranges of the calibration curves (above ~0.5 mRNA copies per human cell based on an assumption of 10 pg of total RNA per cell). System response was linear over more than two orders of magnitude with typical CVs of ~6% for concentrations above 1 fM (10 5 molecules per mL). Profiling the industry-standard MAQC data set yielded correlation coefficients of >0.83 for intensity values and >0.99 for measured ratios. Ninety percent of nCounter™ ratio measurements were within 1.27–1.33 fold changes of the Taqman ® data (0.34–0.41 in log 2 scale) for FF total RNA samples.

          Conclusion

          The nCounter™ Analysis System generated robust data for multi-gene expression signatures across three different sample preparation conditions.

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          Direct multiplexed measurement of gene expression with color-coded probe pairs.

          Gary K Geiss, Roger Bumgarner, Brian Birditt (2008)
          We describe a technology, the NanoString nCounter gene expression system, which captures and counts individual mRNA transcripts. Advantages over existing platforms include direct measurement of mRNA expression levels without enzymatic reactions or bias, sensitivity coupled with high multiplex capability, and digital readout. Experiments performed on 509 human genes yielded a replicate correlation coefficient of 0.999, a detection limit between 0.1 fM and 0.5 fM, and a linear dynamic range of over 500-fold. Comparison of the NanoString nCounter gene expression system with microarrays and TaqMan PCR demonstrated that the nCounter system is more sensitive than microarrays and similar in sensitivity to real-time PCR. Finally, a comparison of transcript levels for 21 genes across seven samples measured by the nCounter system and SYBR Green real-time PCR demonstrated similar patterns of gene expression at all transcript levels.
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            Expression profiling using microarrays fabricated by an ink-jet oligonucleotide synthesizer.

            Timothy Hughes, Mao Mao, Allan Jones (2001)
            We describe a flexible system for gene expression profiling using arrays of tens of thousands of oligonucleotides synthesized in situ by an ink-jet printing method employing standard phosphoramidite chemistry. We have characterized the dependence of hybridization specificity and sensitivity on parameters including oligonucleotide length, hybridization stringency, sequence identity, sample abundance, and sample preparation method. We find that 60-mer oligonucleotides reliably detect transcript ratios at one copy per cell in complex biological samples, and that ink-jet arrays are compatible with several different sample amplification and labeling techniques. Furthermore, results using only a single carefully selected oligonucleotide per gene correlate closely with those obtained using complementary DNA (cDNA) arrays. Most of the genes for which measurements differ are members of gene families that can only be distinguished by oligonucleotides. Because different oligonucleotide sequences can be specified for each array, we anticipate that ink-jet oligonucleotide array technology will be useful in a wide variety of DNA microarray applications.
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              Author and article information

              Journal
              Journal ID (nlm-ta): BMC Res Notes
              Title: BMC Research Notes
              Publisher: BioMed Central
              ISSN (Electronic): 1756-0500
              Publication date Collection: 2009
              Publication date (Electronic): 9 May 2009
              Volume: 2
              Page: 80
              Affiliations
              [1 ]Rosetta Inpharmatics, LLC, 401 Terry Ave N, Seattle, WA 98109, USA
              [2 ]Merck & Co Inc., West Point, PA 19486, USA
              [3 ]NanoString Technologies, 530 Fairview Ave N, Seattle, WA 98109, USA
              [4 ]Novo Nordisk, 530 Fairview Ave N, Seattle, WA 98109, USA
              Article
              Publisher ID: 1756-0500-2-80
              DOI: 10.1186/1756-0500-2-80
              PMC ID: 2688518
              PubMed ID: 19426535
              SO-VID: b4ad5be4-c37b-46ca-962a-f1d9429f1c14
              Copyright © Copyright © 2009 Malkov et al; licensee BioMed Central Ltd.
              License:

              This is an Open Access article distributed under the terms of the Creative Commons Attribution License ( http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

              History
              Date received : 3 September 2008
              Date accepted : 9 May 2009
              Categories
              Subject: Technical Note

              ScienceOpen disciplines: Medicine
              Data availability:
              ScienceOpen disciplines: Medicine

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