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Series GSE26530 Query DataSets for GSE26530
Status Public on Dec 20, 2011
Title Digital gene expression profiling of primary acute lymphoblastic leukemia cells
Organism Homo sapiens
Experiment type Expression profiling by high throughput sequencing
Summary We determined the genome-wide digital gene expression (DGE) profiles of primary acute lymphoblastic leukemia (ALL) cells from 28 patients and fractionated blood cells from healthy blood donors taking advantage of “second generation” sequencing technology. The patients included in the study represent distinct subtypes of B-cell precursor (BCP) ALL and T-cell lineage ALL (T-ALL) and the controls are fractionated CD19+ and CD3+ cells.
 
Overall design Gene expression analysis of 28 ALL patient samples with different immunophenotypic backgrounds including T-ALL (n=4) and patients with BCP ALL with diverse cytogenetic backgrounds: High Hyperploidy (HeH) (n=10), t(9;22) BCR-ABL1 (n=3), t(12;21) ETV6-RUNX1 (n=4), dic(9;20) (n=3), t(1;19)TCF3-PBX1, MLL/11q23 (n=1) and undefined/non-recurrent aberrations (n=1).

Fractionated b-cells (CD19+) and t-cells (CD3+) isolated from peripheral blood of healthy donors were used as controls.

Sequencing libraries were prepared from 1 µg of total RNA using reagents from the NlaIII Digital Gene Expression Tag Profiling kit (Illumina Inc, San Diego, CA, USA). mRNA was captured on magnetic oligo(dT) beads and reverse transcribed into double-stranded cDNA. The cDNA was cleaved using the restriction enzyme NlaIII. An adapter sequence containing the recognition sequence for the restriction enzyme MmeI was ligated to the NlaIII cleavage sites. The adapter-ligated cDNA was digested with MmeI to release the cDNA from the magnetic bead, while leaving 17 base-pairs of sequence in the fragment. The fragments were dephosphorylated and purified by phenol-chloroform. A second adapter was ligated at the MmeI cleavage sites. The adapter-ligated cDNA fragments were amplified by PCR, and the PCR products were purified on a 6% polyacrylamide gel. The ~96 base pair PCR products were excised from the gel and eluted overnight, followed by ethanol precipitation and re-suspension. Purified libraries were quality controlled and quantified on a Bioanalyzer using DNA 1000 series or High Sensitivity chips. The DGE libraries were diluted to a 10 nM concentration and sequenced on one lane of an Illumina GAII or GAIIx for 18 cycles.
 
Contributor(s) Nordlund J, Syvänen A
Citation(s) 22173241, 24063430
Submission date Jan 10, 2011
Last update date May 15, 2019
Contact name Jessica Nordlund
E-mail(s) [email protected]
Phone +46186114912
Organization name Uppsala University
Department Medical Sciences
Lab Molecular Medicine
Street address Academic Hospital, Entrance 70, 3rd floor
City Uppsala
ZIP/Postal code 75185
Country Sweden
 
Platforms (2)
GPL9115 Illumina Genome Analyzer II (Homo sapiens)
GPL10999 Illumina Genome Analyzer IIx (Homo sapiens)
Samples (36)
GSM652276 DGE_dic9-20_1
GSM652277 DGE_dic9-20_2
GSM652278 DGE_dic9-20_3
This SubSeries is part of SuperSeries:
GSE26878 Digital gene and expression profiling of primary acute lymphoblastic leukemia (ALL) cells
Relations
SRA SRP005279
BioProject PRJNA142169

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Series Matrix File(s) TXTHelp

Supplementary file Size Download File type/resource
GSE26530_DGE_Antisense_GeneExpression_TPM.txt.gz 432.3 Kb (ftp)(http) TXT
GSE26530_DGE_RawTagExp_Normalized.txt.gz 19.7 Mb (ftp)(http) TXT
GSE26530_DGE_Sense_GeneExpression_TPM.txt.gz 1.1 Mb (ftp)(http) TXT
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Raw data are available in SRA
Processed data are available on Series record

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