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Sample GSM2845441 Query DataSets for GSM2845441
Status Public on Apr 07, 2018
Title PDX tumor B
Sample type RNA
 
Source name PDX tumor
Organism Homo sapiens
Characteristics host organism: Mus musculus
tissue: patient-derived xenograft (PDX)-derived tumor
original tumor type: triple negative inflammatory breast cancer
Treatment protocol To compare the molecular signatures, we utilized magnetic 3D bio-printing (n3D BiosciencesTM, Inc.). Briefly, viable cells released from the PDX tumor and tagged with poly-L-lysine–tagged magnetic nanoparticle assembly for 24hr were harvested and dispensed into a 96-well ultra-low attachment tissue culture plate at a concentration of 50,000 cells per well, and the plate was placed on a 96 well magnetic bioprinter. Well-formed and equally sized PDXEx “bio-prints” were observed at 5 days of incubation, a time corresponding to the duration of the planned high-throughput drug screens.
Growth protocol Cells harvested from IBC PDX tumors were incubated overnight with poly-L-lysine–covered iron nanoparticles for about 18-24 h at a ratio of 1 µL of nanoshells to 150,000 cells to permit the binding of the iron nanoparticles to the surface of the cells. The nanoparticle-coated cells were then placed in the Bio-Assembler system. Cells were maintained within the Bio-Assembler system for 10 to 14 days at 370C in a humidified environment with medium changed every 3 to 4 days. The best results were obtained from cells released from PDX tumors that were vascular with a fat content between 20% and 30% of the total tumor weight. Tumors weighing 0.8 gram to 1 gram generally yielded the best results.
Extracted molecule total RNA
Extraction protocol Total RNA isolated from the PDX tumors as well as from the ex vivo tumor tissue after 5 days of growth in culture was purified with the Trizol method (Invitrogen) according to the manufacturer’s instructions
Label biotin
Label protocol The fragmented cDNA was labeled by terminal deoxynucleotidyl transferase using the Affymetrix proprietary DNA labeling reagent, which is covalently linked to biotin.
 
Hybridization protocol Following fragmentation, 5 micrograms of biotin-labeled sense-strand cDNA fragments in 200 µL of hybridization mix was loaded onto a human Clariom D array and hybridized to probes on the array in a GeneChip Hybridization Oven 645 (Affymetrix) for 16 h at 45°C with 60 rpm rotation.
Scan protocol GeneChips were scanned using GeneArray G7 scanner (Affymetrix) and quantified into .CEL files with image and signal intensities.
Description 02_Tumor B_(Clariom_D_Human).CEL(normalized)
Data processing Transcriptome Analysis Console software v4.0 (Affymetrix) was used for probe set summarization and robust multiarray average (RMA) normalization procedures.
 
Submission date Nov 08, 2017
Last update date Apr 07, 2018
Contact name Geoffrey Arthur Bartholomeusz
E-mail(s) [email protected]
Phone 713-792-4158
Organization name UT MD Anderson Cancer Center
Department Experimental Therapeutics
Street address 1901 East Road
City Houston
State/province Texas
ZIP/Postal code 77054
Country USA
 
Platform ID GPL23126
Series (1)
GSE106685 Ex-vivo screening platform to identify tumor-specific therapies

Data table header descriptions
ID_REF
VALUE log2 RMA signal

Data table
ID_REF VALUE
AFFX-BkGr-GC03_st 5.66
AFFX-BkGr-GC04_st 5.3
AFFX-BkGr-GC05_st 5.31
AFFX-BkGr-GC06_st 4.71
AFFX-BkGr-GC07_st 4.09
AFFX-BkGr-GC08_st 3.78
AFFX-BkGr-GC09_st 3.45
AFFX-BkGr-GC10_st 3.13
AFFX-BkGr-GC11_st 2.87
AFFX-BkGr-GC12_st 2.6
AFFX-BkGr-GC13_st 2.34
AFFX-BkGr-GC14_st 2.17
AFFX-BkGr-GC15_st 2.05
AFFX-BkGr-GC16_st 2.05
AFFX-BkGr-GC17_st 2
AFFX-BkGr-GC18_st 2.08
AFFX-BkGr-GC19_st 2.22
AFFX-BkGr-GC20_st 2.26
AFFX-BkGr-GC21_st 2.41
AFFX-BkGr-GC22_st 2.69

Total number of rows: 138745

Table truncated, full table size 3130 Kbytes.




Supplementary file Size Download File type/resource
GSM2845441_02_Tumor_B_Clariom_D_Human_.CEL.gz 22.4 Mb (ftp)(http) CEL
Processed data included within Sample table

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