Reproducible, Quantitative, and Flexible Molecular Subtyping of Clinical DLBCL Samples Using the NanoString nCounter System

Veldman-Jones, Margaret H.; Lai, Zhongwu; Wappett, Mark; Harbron, Chris; Barrett, J. Carl; Harrington, Elizabeth A.; Thress, Kenneth S.

doi:10.1158/1078-0432.ccr-14-0357

Cited by 68 publications

(64 citation statements)

References 34 publications

(44 reference statements)

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“…Encouragingly, the difference in matching fresh and frozen replicates was comparable with that seen with technical replicates. The quantitative correlation was also very robust (11), demonstrating that the nCounter platform can generate high-quality data on FFPE material to enable clinically relevant mRNA gene expression studies. Numerous other publications have independently confirmed this conclusion (1-4).…”

Section: Evaluation Of Sample-associated Variablesmentioning

confidence: 87%

“…The Nanostring Technologies nCounter platform is a relatively new technology and has been used within various clinical and research applications (2)(3)(4)(5)(6)(7)(8)(9)(10)(11)(12)(13). The automated nCounter platform hybridizes fluorescent barcodes directly to specific nucleic acid sequences, allowing for the nonamplified measurement of up to 800 targets within one sample (1,14).…”

Section: Introductionmentioning

confidence: 99%

“…The automated nCounter platform hybridizes fluorescent barcodes directly to specific nucleic acid sequences, allowing for the nonamplified measurement of up to 800 targets within one sample (1,14). A number of papers have shown that the Nanostring platform is comparable with other technologies (11,12,14); however, these studies have not assessed the limit of detection (LOD) and the robustness of the platform, which is essential when evaluating precious clinical trial samples.…”

Section: Introductionmentioning

confidence: 99%

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Evaluating Robustness and Sensitivity of the NanoString Technologies nCounter Platform to Enable Multiplexed Gene Expression Analysis of Clinical Samples

et al. 2015

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Analysis of clinical trial specimens such as formalin-fixed paraffin-embedded (FFPE) tissue for molecular mechanisms of disease progression or drug response is often challenging and limited to a few markers at a time. This has led to the increasing importance of highly multiplexed assays that enable profiling of many biomarkers within a single assay. Methods for gene expression analysis have undergone major advances in biomedical research, but obtaining a robust dataset from low-quality RNA samples, such as those isolated from FFPE tissue, remains a challenge. Here, we provide a detailed evaluation of the NanoString Technologies nCounter platform, which provides a direct digital readout of up to 800 mRNA targets simultaneously. We tested this system by examining a broad set of human clinical tissues for a range of technical variables, including sensitivity and limit of detection to varying RNA quantity and quality, reagent performance over time, variability between instruments, the impact of the number of fields of view sampled, and differences between probe sequence locations and overlapping genes across CodeSets. This study demonstrates that Nanostring offers several key advantages, including sensitivity, reproducibility, technical robustness, and utility for clinical application.

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Section: Evaluation Of Sample-associated Variablesmentioning

confidence: 87%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Evaluating Robustness and Sensitivity of the NanoString Technologies nCounter Platform to Enable Multiplexed Gene Expression Analysis of Clinical Samples

et al. 2015

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“…MicroRNA gene expression was measured using the nCounter Human v1 microRNA Expression Assay (NanoString Technologies, Seattle, WA) (14,31,40). RNA (100 ng) from each biopsy was hybridized with the nCounter probe set.…”

Section: Methodsmentioning

confidence: 99%

Integrative mRNA-microRNA analyses reveal novel interactions related to insulin sensitivity in human adipose tissue

Kirby

Walton

Finlin

et al. 2016

Physiological Genomics

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“…A more targeted, smaller miRNA array was then constructed, lowering the per sample cost and allowing for much larger cohorts to be analyzed in a cost-effective manner in order to validate and refine signatures and biomarkers. The gene expression platform assay system strikes a balance between the traditional exploratory nature of the microarray and more targeted, hypothesis-driven data collection to refine and test molecular signatures and biomarkers [14][15][16] . The method will be used to examine molecular and protein perturbations in in vivo and in vitro models where the described target miRNAs are experimentally over-expressed or inhibited.…”

Section: Future Applications or Directions After Mastering This Technmentioning

confidence: 99%

Perturbations of Circulating miRNAs in Irritable Bowel Syndrome Detected Using a Multiplexed High-throughput Gene Expression Platform

Fourie

Peace

Abey

et al. 2016

JoVE

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The gene expression platform assay allows for robust and highly reproducible quantification of the expression of up to 800 transcripts (mRNA or miRNAs) in a single reaction. The miRNA assay counts transcripts by directly imaging and digitally counting miRNA molecules that are labeled with color-coded fluorescent barcoded probe sets (a reporter probe and a capture probe). Barcodes are hybridized directly to mature miRNAs that have been elongated by ligating a unique oligonucleotide tag (miRtag) to the 3' end. Reverse transcription and amplification of the transcripts are not required. Reporter probes contain a sequence of six color positions populated using a combination of four fluorescent colors. The four colors over six positions are used to construct a gene-specific color barcode sequence. Post-hybridization processing is automated on a robotic prep station. After hybridization, the excess probes are washed away, and the tripartite structures (capture probe-miRNA-reporter probe) are fixed to a streptavidin-coated slide via the biotin-labeled capture probe. Imaging and barcode counting is done using a digital analyzer. The immobilized barcoded miRNAs are visualized and imaged using a microscope and camera, and the unique barcodes are decoded and counted. Data quality control (QC), normalization, and analysis are facilitated by a custom-designed data processing and analysis software that accompanies the assay software. The assay demonstrates high linearity over a broad range of expression, as well as high sensitivity. Sample and assay preparation does not involve enzymatic reactions, reverse transcription, or amplification; has few steps; and is largely automated, reducing investigator effects and resulting in high consistency and technical reproducibility. Here, we describe the application of this technology to identifying circulating miRNA perturbations in irritable bowel syndrome. Video LinkThe video component of this article can be found at

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Reproducible, Quantitative, and Flexible Molecular Subtyping of Clinical DLBCL Samples Using the NanoString nCounter System

Cited by 68 publications

References 34 publications

Evaluating Robustness and Sensitivity of the NanoString Technologies nCounter Platform to Enable Multiplexed Gene Expression Analysis of Clinical Samples

Evaluating Robustness and Sensitivity of the NanoString Technologies nCounter Platform to Enable Multiplexed Gene Expression Analysis of Clinical Samples

Integrative mRNA-microRNA analyses reveal novel interactions related to insulin sensitivity in human adipose tissue

Perturbations of Circulating miRNAs in Irritable Bowel Syndrome Detected Using a Multiplexed High-throughput Gene Expression Platform

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