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Sample GSM1335520 Query DataSets for GSM1335520
Status Public on Feb 27, 2014
Title ML-2
Sample type genomic
 
Source name 5C library from ML-2 cell line
Organism Homo sapiens
Characteristics cell line: ML-2
mll state: AF6
leukemia type: AML
Growth protocol Grown in RPMI 1640 (Gibco) supplemented with 10% FBS (Fisherbrand), and 1% penicillin-streptomycin (Invitrogen™).
Extracted molecule genomic DNA
Extraction protocol 5C libraries were generated by incubating an individual 3C library with a pool of 5C primers to a final volume of 10ul of annealing buffer (20mM tris-acetate pH 7.9, 50mM potassium acetate, 10mM magnesium acetate, and 1mM dithiothreitol), and to final individual primer concentrations of 20nM. 5C primers were annealed to 3C templates overnight at 48ºC, and ligated the following day by adding 20ul of ligation buffer containing 10 units of Taq DNA ligase (NEB; 25mM Tris-HCl pH 7.6, 31.25mM potassium acetate, 12.5mM magnesium acetate, 1.25mM NAD, 12.5mM dithiothreitol, 0.125% Triton X-100) for 1h at 48ºC. The reactions were terminated by a 10 minute incubation at 65ºC.
Label Cy5
Label protocol The 5C libraries were amplified by PCR with the T7 (TAATACGACTCAACTATAGCC) and 5'-Cy3-labelled T3 (TATTAACCCTCACTAAAGGGA) primers, respectively. Unincorporated primers and other contaminants were removed from the 5C libraries using the MinElute Reaction Cleanup kit (Qiagen®).
 
Hybridization protocol As per the manufacturer’s guidelines, approximately 100 ng of 5C library were individually hybridized to arrays using the NimbleGen CGH Hybridization kit.
Scan protocol 5C arrays were scanned with a DNA microarray scanner (Agilent Technologies, model G2505) at 5 µm resolution.
Description Raw feature file from scanning 5C library on microarray and corresponding normalized data
Data processing Raw data were extracted from the images using the NimbleScan 2.6 software (NimbleGen Systems, Inc.), and specific features were extracted with our 'ArrayQC' software and then normalized using our 'Ifcalculator' software.
420 out of over 350,00 probes: 5C data filtered for noise and normalized for both quantity of DNA hybridized (using a gene desert) and primer pair efficiency (using a BAC library)
 
Submission date Feb 26, 2014
Last update date Feb 27, 2014
Contact name Josée Dostie
E-mail(s) josee.dostie@mcgill.ca
Phone 1-514-398-4975
Organization name McGill University
Department Biochemistry
Street address 3655 Promenade Sir-William-Osler
City Montreal
State/province QC
ZIP/Postal code H3G 1Y6
Country Canada
 
Platform ID GPL18341
Series (2)
GSE55406 Classifying leukemia types with chromatin conformation data (5C)
GSE55408 Classifying leukemia types with chromatin conformation data

Data table header descriptions
ID_REF
VALUE 5C data filtered for noise and normalized for both quantity of DNA hybridized (using a gene desert) and primer pair efficiency (using a BAC library)

Data table
ID_REF VALUE
5C_HOXA_F_47_HOXA_R_50_24 3.471750799
5C_HOXA_F_47_HOXA_R_52_24 0.631629182
5C_HOXA_F_47_HOXA_R_54_24 1.906245198
5C_HOXA_F_47_HOXA_R_56_24 1.490127871
5C_HOXA_F_47_HOXA_R_58_24 0.99444084
5C_HOXA_F_47_HOXA_R_60_24 0.988841876
5C_HOXA_F_47_HOXA_R_62_24 0.90291091
5C_HOXA_F_47_HOXA_R_64_24 0.758427001
5C_HOXA_F_47_HOXA_R_66_24
5C_HOXA_F_47_HOXA_R_68_24 1.309111426
5C_HOXA_F_47_HOXA_R_70_24 0.985107086
5C_HOXA_F_47_HOXA_R_72_24 0.78275547
5C_HOXA_F_47_HOXA_R_74_24 0.516038421
5C_HOXA_F_47_HOXA_R_76_24 0.668623517
5C_HOXA_F_47_HOXA_R_78_24 0.773341004
5C_HOXA_F_47_HOXA_R_80_24 0.461601136
5C_HOXA_F_47_HOXA_R_82_24 0.447660939
5C_HOXA_F_47_HOXA_R_84_24 0.69721731
5C_HOXA_F_47_HOXA_R_86_24 0.629843024
5C_HOXA_F_47_HOXA_R_88_24 0.563030995

Total number of rows: 420

Table truncated, full table size 14 Kbytes.




Supplementary file Size Download File type/resource
GSM1335520_ML-2.ftr.gz 6.3 Mb (ftp)(http) FTR
Processed data included within Sample table

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