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Sample GSM5946560 Query DataSets for GSM5946560
Status Public on May 08, 2024
Title 2A_YUPEET [RPPA]
Sample type protein
 
Source name melanoma cell line_YUPEET
Organism Homo sapiens
Characteristics gender: M
age at diagnosis: 54
cohort: Yale
cell type: primary cutaneous melanoma tissue
Treatment protocol N/A
None
Growth protocol This cohort includes human cell lines (n=5, in triplicate). WM35, WM983, and WM1552c were grown in 2% tumor media containing a 4:1 mixture of MCDB 153 medium with 1.5 g/L sodium bicarbonate and Leibovitz's L-15 medium with 2 mM L-glutamine supplemented with 0.005 mg/ml bovine insulin, 1.68 mM CaCl2, and 2% fetal bovine serum. . YUPEET and YUCHIME were grown in bFGF media (OPTIMEM, 5% FBS, 10ng/ml bFGF, 1ng/ml heparin, 0.1mM dbcAMP, 0.1mM IBMX.)
This cohort includes human tissue obtained from FFPE (n=205), fresh frozen human tissue (n=24), and human cell lines (n=12).
Extracted molecule protein
Extraction protocol Cell were lysed using lysis Buffer (1% Triton X‐100, 50mM HEPES, pH 7.4, 150mM NaCl, 1.5mM MgCl2, 1mM EGTA, 100mM NaF, 10mM Na pyrophosphate, 1mM Na3VO4, 10% glycerol, containing freshly added protease and phosphatase inhibitors) for 30 minutes while shaking. The cell lysates were centrifuged at 14,000 rpm for 10 minutes at 4C. Supernatant was collected, pellet discarded. Protein concentration was quantified by Qubit and adjusted to 1.5 ug/ul. (using lysis buffer to dilute). The cell lysate was mixed with (4XSDS + B‐Me) sample buffer without bromophenol blue (3 parts of cell lysate plus one part of 4XSDS sample buffer). The samples were boiled for 5 minutes, and stored in –80C until sample submission.
RNA was obtained from the FFPE human tissue samples using the RecoverAll Total Nucleic Acid Isolation kit. RNA was obtained from the fresh frozen human tissue samples using the Qiagen Rneasy kit. Cell lines were pelleted and RNA was harvested using the Qiagen Rneasy kit.
Label NA
Label protocol NA
Specimens were labeled with decode assignment which was linked to tumor origin.
 
Hybridization protocol Serially diluted cellular proteins are arrayed on nitrocellulose‐coated slides and probed with validated antibodies that recognize signaling molecules in their functional state. Signals are captured by tyramide dye deposition and a DAB colorimetric reaction.
200 ng RNA was hybridized to a custom NanoString panel code set according to the recommendations of the manufacturer (NanoString Technologies, Inc., Seattle, Washington, USA).
Scan protocol Data is collected and quantitative analysis is performed using custom “Supercurve”software developed for this purpose. The values derived from the slope and intercept are expressed relative to standard control cell lysates or control peptides on the array. Thesevalues indicate the levels of protein expression and modification (phosphorylation or cleavage based on antibody specificity)
Following hybridization, the target-probe complexes were purified and immobilized on the nCounter prep station. Digital counts for each gene-specific target RNA were then acquired on the nCounter detection analyzer and normalized to account for differences in tissue mRNA quantity as well as slight differences in assay efficiency.
Data processing Each dilution curve was fitted with a logistic model (“Supercurve Fitting” developed by the Department of Bioinformatics and Computational Biology in MD Anderson Cancer Center, “http://bioinformatics.mdanderson.org/OOMPA”). This fits a single curve using all the samples (i.e., dilution series) on a slide with the signal intensity as the response variable and the dilution steps are independent variable. The fitted curve is plotted with the signal intensities – both observed and fitted ‐ on the y‐axis and the log2‐concentration of proteins on the x‐axis for diagnostic purposes. The protein concentrations of each set of slides were then normalized for protein loading. Correction factor was calculated by: 1) median‐centering across samples of all antibody experiments; and 2) median‐centering across antibodies for each sample.
The nSolver analysis software version 4.0 (NanoString Technologies) was used for extraction of raw digital counts of expression, checking the quality of the data, normalizing expression values using housekeeping genes, and generating heatmaps.
 
Submission date Mar 11, 2022
Last update date May 08, 2024
Contact name Tiphaine Christiane Martin
E-mail(s) [email protected]
Phone 2128248403
Organization name Icahn School of Medicine at Mount Sinai, Tisch Cancer Institute
Department Oncological Sciences
Lab Parsons
Street address 1470 Madison Ave
City New York
State/province 75459
ZIP/Postal code 10029
Country USA
 
Platform ID GPL32054
Series (2)
GSE198428 An epigenetic gene signature underlies phenotype switching in early stage melanomas [RPPA]
GSE198432 An epigenetic gene signature underlies phenotype switching in early stage melanomas.

Data table header descriptions
ID_REF
VALUE Normalized log2 Median Centered

Data table
ID_REF VALUE
14-3-3-beta-R-V -0.022155065
14-3-3-zeta-R-V 0.112554393
4E-BP1-R-V -0.110876477
4E-BP1_pS65-R-V -0.042712008
53BP1-R-V 0.154401639
A-Raf-R-V -0.043783002
ACC1-R-C 0.194603858
ACC_pS79-R-V 0.097584058
ADAR1-M-V 0.112363759
Akt-R-V 0.310117523
Akt_pS473-R-V -0.316688878
Akt_pT308-R-V -0.604719839
AMPK-a2_pS345-R-V 0.049429711
AMPKa-R-C 0.000639174
AMPKa_pT172-R-C 0.395931824
Annexin-I-M-V -1.047856156
Annexin-VII-M-V 0.072777461
AR-R-V -0.375315181
ARID1A-R-C -0.079366341
Atg3-R-V 0.314303794

Total number of rows: 306

Table truncated, full table size 7 Kbytes.




Supplementary data files not provided
Processed data included within Sample table

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