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Sample GSM7980110 Query DataSets for GSM7980110
Status Public on Sep 27, 2024
Title Tepotinib-treated, ROI 078
Sample type protein
 
Source name METex14 NSCLC
Organism Homo sapiens
Characteristics Sex: female
tumor type: NSCLC
mutation: METex14
tnm: ypT1aN0M0
ttf1 staining: negative
tissue: Periphery
Treatment protocol The slide preparation was performed as per GeoMx DSP Slide Preparation Protocol using the Semi-Automated BOND Rx protocol. In brief, 5 µm tissue sections were positioned in the GeoMx imaging area on a SuperFrost Plus slide. Sections were incubated at 60 ˚C for over 30 minutes prior to BOND Rx protocol. BOND Rx protocol consisted of Bake & Dewax, HIER for 20 minutes with ER1.
Growth protocol FFPE blocks, tepotinib-treated surgical resection was obtained following 42 days of tepotinib treatment
Extracted molecule protein
Extraction protocol n.a.
Label n.a.
Label protocol Following BOND Rx protocol, slides were incubated overnight at 37 ˚C with the selected protein panels: Immune Cell Profiling, Immune Cell Typing, Immune Activation Status, IO Drug Targets, PI3K/AKT Signaling; as well as the morphology markers: TTF1, CD3 and CD33. The following day, post-fixation of section was performed, after washing the slides 3 times in TBS-T for 10 minutes, using 4% paraformaldehyde in a humidity chamber for 30 minutes. Slides were then washed twice for 2 minutes in TBS-T. Nuclear staining was then performed in a humidity chamber using SYTO13 DNA stain for 15 minutes. Slides were finally washed twice in TBS-T before being loaded into the GeoMx DSP instrument.
 
Hybridization protocol n.a.
Scan protocol Scanned using the GeoMx DSP (NanoString Technologies)
Description 20231006_P1001660003346A_P1001660003346A_09.RCC
DNA barcode cleaved from RNA probe
Data processing For an nCounter readout, the collected samples were first hybridized overnight to the GeoMx Hyb Code master mixes, consisting of probes U and R in hybridization buffer, as outlined in the GeoMx nCounter protein readout user guide. Hybridization products were then pooled for readout on the MAX/FLEX nCounter system. RCC files were loaded back onto the GeoMx instrument for downstream analysis in the GeoMx Analysis Suite.
 
Submission date Dec 18, 2023
Last update date Sep 27, 2024
Contact name Manon A Simard
E-mail(s) [email protected]
Organization name Merck Healthcare KGaA
Department Research Unit Oncology
Street address Frankfurterstraße 250
City Darmstadt
ZIP/Postal code 64293
Country Germany
 
Platform ID GPL34024
Series (1)
GSE250509 Protein expression from paired biopsies from a patient with METex14 skiping non-small cell lung cancer before and after treatment with neoadjuvant tepotinib (42 days)

Data table header descriptions
ID_REF
VALUE Results were obtained after processing of the nCounter RC files using the GeoMx Analysis Suite. First, quality check (QC) was performed with a binding QC density of 0.1-2.25, positive control normalization factor QC of 0.3-3.0, 75% of fields of view (FOV) detected, minimum surface area QC threshold of 1600 µm^2, and minimum nuclei count threshold of 20. This was followed by normalization using the metric mean of the Ms IgG1 and Rb IgG as negative controls, selected for normalization after comparing normalization methods using the Evaluate normalization custom script, available through NanoString.

Data table
ID_REF VALUE
Ki-67 148.9445379
CD68 544.4138
CTLA4 16.04307347
CD11c 241.6089917
CD8 418.8325707
Beta-2-microglobulin 271.1220698
S6 5911.71879
CD45 1978.083738
Ms IgG1 68.42953296
HLA-DR 4034.117226
GZMB 278.1697687
GAPDH 1866.338913
SMA 14972.45587
PD-L1 28.61543818
Fibronectin 19515.92872
PanCk 1679.526084
CD20 119.7623053
CD4 416.5604774
Ms IgG2a 83.04839708
PD-1 88.74810589

Total number of rows: 58

Table truncated, full table size 1 Kbytes.




Supplementary data files not provided

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