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Sample GSM2865993 Query DataSets for GSM2865993
Status Public on Nov 28, 2017
Title 9270006104_I; T-PLL
Sample type RNA
 
Source name PATIENT_ID: 478-002_
Organism Homo sapiens
Characteristics cell type: T-PLL
sampleID: 478-002_
caseid: TP032
tcl1a: NEG
mtcp1: NA
os_diagnosis_to_last_fu: 1088
os_treatment_to_last_fu: NA
os_scoring: AWD
pfs: NA
pfs_scoring: alive in ongoing CR or PR
wbc_diagn: 18
wbc_sample: 21
Extracted molecule polyA RNA
Extraction protocol GEP of human T-PLL cells. Sample preparation: PBMCs isolated from T-PLL patients (>95% purity of T-cells) and CD3+ T-cells isolated from PB of healthy donors (see paragraph 2 for detailed descriptions on cell purification) were submitted to RNA isolation using the mirVana kit (Invitrogen). GEP analyses were conducted using Illumina HumanHT‑12 v4 BeadChip arrays according to manufacturer’s instructions.
Label Cy3
Label protocol Standard Illumina protocol
 
Hybridization protocol Standard Illumina hybridization protocol
Scan protocol Standard Illumina scanning protocol
Description NA
9270006104_I
Data processing Bioinformatics: We used the Illumina proprietary software GenomeStudio v1 to background-correct and to initially annotate the probes of the HumanHT-12 v4 Expression BeadChip. We filtered samples and genes by detection p-values and fluorescence intensities for at least 2/3 hits (p<0.05) to reduce false calls. Batch-effects were corrected by the ComBat method which uses an empiric Bayesian model framework. For literature references to bioinformatics methods and algorithms see Supplementary Table2). Since the official Illumina HumanHT-12 v4 Expression BeadChip annotation is outdated, we used the data mining tool biomaRt, version 75 of the Ensembl data base with R, version 3.1.0, and Bioconductor, version 2.10.
T-PLLs (n=70) and normal controls (CD3+ T-cells from 10 healthy donors) were grouped and tested separately for differential expression using the Student’s t-test on log-transformed fluorescence values (normally distributed). Fold-changes (fc) were calculated on the fluorescence values without logarithmic transformation. False discovery rates (FDRs) were calculated using the R package “qvalue”. Hierarchical clustering was carried out using the R package gplots, version 2.15.0 (distance function: euclidean; clustering: complete linkage).
 
Submission date Nov 27, 2017
Last update date Jan 23, 2018
Contact name Giuliano Crispatzu
Organization name University of Cologne (UoC), Germany
Department CECAD
Street address Joseph-Stelzmann-Straße 26
City Cologne
ZIP/Postal code 50931
Country Germany
 
Platform ID GPL10558
Series (2)
GSE107397 The molecular basis of T-PLL is an actionable perturbation of TCL1/ATM- and epigenetically instructed damage responses [human gene expression array]
GSE107513 The molecular basis of T-PLL is an actionable perturbation of TCL1/ATM- and epigenetically instructed damage responses

Data table header descriptions
ID_REF
VALUE normalized

Data table
ID_REF VALUE
ILMN_1762337 4.92803370223572
ILMN_2055271 6.01553202626259
ILMN_1736007 4.60279298189627
ILMN_2383229 5.48756588066512
ILMN_1806310 5.04044723174436
ILMN_1779670 4.64898255582241
ILMN_1653355 4.87482844054292
ILMN_1717783 3.3631874070026
ILMN_1705025 4.68968462235306
ILMN_1814316 5.27700699439269
ILMN_2359168 4.84930256368317
ILMN_1731507 3.63464362487942
ILMN_1787689 5.08030167169025
ILMN_3241953 6.47383259868614
ILMN_1745607 4.31980966702992
ILMN_2136495 4.76413483908746
ILMN_1668111 4.53483723311654
ILMN_2295559 4.42711196130548
ILMN_1735045 4.3362632680709
ILMN_1680754 5.36552234477493

Total number of rows: 47293

Table truncated, full table size 1380 Kbytes.




Supplementary file Size Download File type/resource
GSM2865993_9270006104_I_Grn.idat.gz 1.6 Mb (ftp)(http) IDAT
Processed data included within Sample table

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