NCBI Logo
GEO Logo
   NCBI > GEO > Accession DisplayHelp Not logged in | LoginHelp
GEO help: Mouse over screen elements for information.
          Go
Sample GSM6068357 Query DataSets for GSM6068357
Status Public on Sep 28, 2022
Title Pre patient 19 [Sample 50]
Sample type RNA
 
Source name primary high grade serous ovarian cancer
Organism Homo sapiens
Characteristics tissue: primary high grade serous ovarian cancer biopsy
histology: high grade serous ovarian cancer
Stage: IIIC
Sex: female
age: 75
platinum-free interval: 7
progression status as of 4/25/22: yes
Treatment protocol patients samples were obtained from naïve tumors during biopsy, or during interval debulking sugery after neoadjuvant treatment with carboplatin and paclitaxel chemotherapy
Extracted molecule total RNA
Extraction protocol Pre-treatment and post-treatment cases were reviewed to select an optimal formalin-fixed, paraffin-embedded tissue block for each case. An optimal pre-treatment block contained maximum tumor cellularity (minimum of 20%) with no lymph node tissue present. An optimal post-treatment block contained maximum tumor cellularity (minimum of 20%) with no lymph node tissue present, and with evidence of a lymphocytic response. For each block, ten unstained sections of 4-5 micron thickness were cut and placed on Avantix uncharged slides. An eleventh slide was cut at 4-5 microns, stained with hematoxylin and eosin, cover-slipped and reviewed to confirm the appropriate tissue was still present. FFPE sections were scraped into tubes for RNA isolation using an RNeasy FFPE Kit (Qiagen, 73504) according to manufacturer’s instructions. RNA concentration and quality was measured by NanoDrop
Label fluorescent barcode
Label protocol n/a
 
Hybridization protocol The reporter code set and capture probe set tubes were removed from -80C and thawed on ice, prior to mixing by tapping and pulse centrifugation. 70 µl hybridization buffer was added to the tube containing the reporter probe set and mixed by tapping, followed by pulse centrifugation. 8 µl of the diluted reporter probe was added to a PCR tube. Each RNA sample was diluted in water to 25 ng/µl and 2 µl final volume for 50 ng total input per sample. 5 µl RNA sample was added to each tube containing the reporter probe set and mixed by tapping, followed by pulse centrifugation. 2 µl Capture Probe Set was added to each tube, mixed by tapping, and the sample was collected by pulse centrifugation and then immediately placed in a pre-heated PCR machine, with the lid set to 70 °C and the block set to 65 °C. The hybridization was performed for 18 h at 65 °C. Samples were cooled to 4 °C and any condensation was collected by pulse centrifugation. Each sample was diluted with 18 µl hybridization buffer.
Scan protocol An nCounter Sprint cartridge was calibrated to room temperature for 15 min prior to injection of 33 µl of each sample into one of the 12 injection ports of the cartridge, followed by the introduction of an air seal. The sample injection cartridge was sealed with provided tape and the reagent supply ports were unsealed prior to loading on the nCounter Sprint profiler. The analysis run was started immediately after loading.
Description low count genes were filtered out for a total of 750 genes detected on the panel
Data processing The resulting data file in RCC format was used for data analysis in the nCounter Advanced Analysis Software. Raw data in RCC format was uploaded to nSolver for automated normalization, background subtraction, and quality control (QC) check.
 
Submission date Apr 26, 2022
Last update date Sep 28, 2022
Contact name Jennifer Renee Ribeiro
E-mail(s) [email protected]
Organization name Women and Infants Hospital of Rhode Island
Department Obstetrics and Gynecology
Street address 200 Chestnut St.
City Providence
State/province RI
ZIP/Postal code 02903
Country USA
 
Platform ID GPL27956
Series (1)
GSE201600 Immunologic adapatations of high grade serous ovarian cancer patients to neoadjuvant carboplatin and paclitaxel therapy

Data table header descriptions
ID_REF
VALUE log2 normalized mRNA counts

Data table
ID_REF VALUE
CCNO 4.133812954
MYC 8.65737491
CD79A 4.133812954
FSTL3 7.326458032
VCAN 11.15618077
CX3CL1 6.611860251
ERBB2 8.315142719
FAM124B 5.133812954
AKT1 9.332082581
KDR 6.413920873
EGF 1.326458032
MAGEA12 4.326458032
IFNA1 2.326458032
TGFB3 8.486329369
MFGE8 10.7548182
CXCL2 6.455741049
CCND2 8.526130377
PDZK1IP1 4.785889651
JAG2 4.496383033
C5 5.574385545

Total number of rows: 750

Table truncated, full table size 13 Kbytes.




Supplementary file Size Download File type/resource
GSM6068357_20220216_30102684500922-01_Sample06_06.RCC.gz 8.5 Kb (ftp)(http) RCC
Processed data included within Sample table
Processed data are available on Series record

| NLM | NIH | GEO Help | Disclaimer | Accessibility |
NCBI Home NCBI Search NCBI SiteMap