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Sample GSM7384851 Query DataSets for GSM7384851
Status Public on Jan 25, 2024
Title human_RLT_region_120
Sample type SRA
 
Source name reactive lympoid tissues
Organism Homo sapiens
Characteristics tissue: reactive lympoid tissues
region cell_type: CD20
Extracted molecule total RNA
Extraction protocol The slides were incubated with blocking Buffer W (200 ?L/slide, NanoString) for 30 min in the humidity chamber at room temperature after hybridization.Each slide was stained with corresponding morophology markers. After immunofluorescent staining, the slides were visualized using the GeoMx® DSP instrument to select regions of interest (ROIs). To acquire representative regions, ROI selection was performed by an expert pathologist. The pathologist was blinded to the group assignment during the ROIs selection. Based on fluorescent staining, each ROI was segmented into corresponding areas of interest (AOIs) - CD68+ regions, CD3+ regions, and CD20+ regions. Subsequently, each AOI was exposed to UV light and photocleaved oligos were aspirated from the solution into the wells of a collection plate.
Collected photocleaved oligos were PCR amplified with the corresponding GeoMx® Seq Code Primer Plate and Master Mix (NanoString). PCR products were pooled and cleaned with AMPure XP beads (Agilent, Santa Clara, California, USA) twice to obtain the libraries. The quality and concentration of libraries were assessed using a high sensitivity DNA Kit (Agilent) and Bioanalyzer. Subsequently, libraries were sequenced on an illumina sequencing platform (Hiseq or NovaSeq) with standard workflow specifications (dual-indexing and paired-end reads (2?×?27?bp)).
 
Library strategy RNA-Seq
Library source transcriptomic
Library selection cDNA
Instrument model Illumina NovaSeq 6000
 
Description Tonsil1+2 CD3CD20CD68|031|CD20
Data processing The GeoMx® NGS Pipeline is used to process FASTQ sequencing files from Nanostring GeoMx libraries to produce digital count conversion (.dcc) files. Once complete, all DCC files are packed into a zip file and available to download. This zip file can be uploaded into the GeoMx Digital Spatial Profiler (DSP) system for quality control and normalizaton.
Raw reads were trimmed, stitched, aligned, and deduplicated to transform digital counts data with unique targets. AOIs with fewer than 10,000 raw reads or sequencing saturation <50% were filtered out of the analysis. AOIs with less than 5% of all target genes (18,000+) and target genes that do not achieve the limit of quantitation were removed. The data was then processed with the Q3 normalization method for all the remaining targets. Q3 normalization divides the counts in one segment by the 3rd quartile value for that segment, then subsequently multiplies that value by the geometric mean of the 3rd quartile values of all segments. Q3 normalization rescales the gene expression data such that all segments have similar gene expression ranges. It reduces variance from segment size, segment cellularity, and other technical factors. Underlying the Q3 method is an assumption that, despite biological variation, segments should have similar gene expression count distributions. Thus, Q3 is only appropriate when a probe panel is large and diverse, such as one that targets the full transcriptome.
Assembly: hg38
Supplementary files format and content: The file named processed data (DSP_gene_matrix) showed the genes expression of all DLBCL tissues and 12 tonsil samples, sequencing by illimina hiseq3000.
Supplementary files format and content: The file named processed data2 (DSP_gene_matrix) showed the genes expression of the rest of tonsil samples, sequencing by illimina novaseq 6000.
 
Submission date May 18, 2023
Last update date Jan 25, 2024
Contact name Min Liu
E-mail(s) liuminnus@gmail.com
Organization name National University of Singapore
Street address 13-02, 14 Medical Drive, Singapore
City Singapore
ZIP/Postal code 117599
Country Singapore
 
Platform ID GPL24676
Series (1)
GSE232853 Spatially-resolved transcriptomics reveal macrophage heterogeneity and prognostic significance in diffuse large B-cell lymphoma
Relations
BioSample SAMN35165623
SRA SRX20437100

Supplementary data files not provided
SRA Run SelectorHelp
Raw data are available in SRA
Processed data are available on Series record

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