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SRX383201: GSM1274535: MCIC4; Homo sapiens; RNA-Seq
4 ABI_SOLID (AB 5500xl Genetic Analyzer) runs: 36.3M spots, 1.8G bases, 1.1Gb downloads

Submitted by: Gene Expression Omnibus (GEO)
Study: Flexible multiplatform RNA profiling at the single cell level applied to enriched cancer initiating cells: RNA-Seq CIC data
show Abstracthide Abstract
Accurate profiling of RNA expression of single cells is a valuable approach for broadening our understanding of cancer biology and mechanisms of dissemination, but requires the development of reliable methods for their molecular characterization. Here we evaluate a single cell methodology which generates microgram amounts of cDNA suitable for next generation sequencing (RNA-Seq), high throughput RT-qPCR and Affymetrix array analysis. The approach was tested by comparing expression profiles of amplified single MCF7 and MCF10A cells to profiles generated from unamplified RNA. The expression profiles were compared by Affymetrix-U133 arrays, RNA-Seq and high-density qPCR. There were strong cross-platform correlations of >80% and concordance between single cell and unamplified material of >70%. We exemplify the approach through analysis of rare sorted cancer initiating cells (CICs) derived from a NSCLC patient-derived xenograft. Populations of 10 cells from total tumour and two distinct subsets of CIC, putatively involved in primary tumor maintenance or metastasis formation were FACS sorted then directly amplified. CIC expression profiles strongly correlated with published stem-cell and epithelial-mesenchymal transition (EMT) signatures. Our results confirm the utility of the amplification system and our methodology to detect and distinguish RNA profiles in rare cell populations that inform on EMT and stem-cell characteristics. This GEO dataset comprises the RNA-Seq data for total tumour, MCIC and RCIC samples. Overall design: 12 samples. 4 biological replicates each of total tumour cDNA generated from amplified RNA from a volume equivalent to 10 single cells, metastasis associated cancer-initiating cell cDNA generated from amplified RNA from a volume equivalent to 10 single cells, and resident cancer initiating cell cDNA generated from amplified RNA from a volume equivalent to 10 single cells. RNA-Seq data for these 3 groups (total tumour, metastasis associated cancer initiating cells and resident cancer initiating cells) were compared.
Sample: MCIC4
SAMN02420393 • SRS507280 • All experiments • All runs
Organism: Homo sapiens
Library:
Instrument: AB 5500xl Genetic Analyzer
Strategy: RNA-Seq
Source: TRANSCRIPTOMIC
Selection: cDNA
Layout: PAIRED
Construction protocol: To obtain single cell suspension, PDXs were mechanically and then enzymatically digested in a solution of collagenase IV (5mg/ml) and DNase (100U/ml) (Sigma-Aldrich) in DMEM/F12 (Lonza) for 1h at 37 °C. Partially digested tissue was filtered through a 100µm cell strainer (BD Falcon) and red blood cells were removed by Lysing Buffer 1X (BD Bioscience). Single cell suspensions from dissociated NSCLC-PDXs were washed and incubated in staining solution 1% BSA and 2mM EDTA with specific antibodies at appropriate dilutions for 30 min at 4 °C: PE anti-human CD133/1, FITC anti-human CD326 (EpCAM) (Miltenyi Biotech), APC anti-human CD187 (CXCR4) (BD Pharmingen), Alexa Fluor® 488 anti-human HLA-ABC (BD Pharmingen) , PerCP-eFluor 710 anti-mouse MHC class I (e-Bioscience). Prior to sorting, cells were resuspended to a final concentration of 10x106 cells/ml in Hepes Buffered Saline (HBS) (Lonza) + 0.1% B27 Supplements (Gibco) and 7-AAD viability staining solution (1:10) (e-Bioscience) for dead cells exclusion. PDX-cells were sorted with FACSAria (Becton Dickinson) into a chilled 96-well plate (Corning Incorporated). For sorting of different CSC fractions, an initial gate excluding doublets, dead cells and mouse MHC class I+ cells was set. Then, within the gate of human viable CD133+ cells, the fraction of EpCAM+ and CXCR4+EpCAM- cells were identified and sorted. Total tumor population was isolated based on human HLA-ABC+ expression. For each cell fraction, 300 cells were directly sorted in 30 μl of CLS (Complete Lysis Solution) per well and within 1h approximately 100 cells/10 μl were transferred into 0.5 ml tubes and stored to -80 0C. To ensure all cDNA generated using the Epistem RNA Amp kit was double stranded one cycle of re-amplification was performed. RNA (1ng-25pg) or cell lysates in CLS were adjusted to 6.75ml volume and RNA-amplified using the EpiStem RNA-Amp Kit according to the manufacturers protocols (EpiStem, Manchester, UK). Briefly the samples underwent oligo-dT priming and 5’ capping prior to x35 cycles of PCR amplification using the conditions 90ºC 30 sec, 42ºC 2 min and 72ºC 6 min. Following amplification all samples were purified using a MoBio UltraClean® PCR Clean-Up Kit (Carlsbad, CA, USA) and quantified on a NanoDrop spectrophotometer.
Experiment attributes:
GEO Accession: GSM1274535
Links:
External link:
Runs: 4 runs, 36.3M spots, 1.8G bases, 1.1Gb
Run# of Spots# of BasesSizePublished
SRR10376658,589,332429.5M267.4Mb2014-12-31
SRR10376669,061,599453.1M284.7Mb2014-12-31
SRR12661288,936,541446.8M279.7Mb2014-12-31
SRR12661299,680,915484M314.2Mb2014-12-31

ID:
547970

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