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SRX15542602: GSM6208863: Mouse intestinal crypt epithelial cells from adult male C57BL/6J (8 weeks old), untreated, scRNA-seq; Mus musculus; RNA-Seq
1 ILLUMINA (Illumina NovaSeq 6000) run: 413.9M spots, 41.8G bases, 11.2Gb downloads

External Id: GSM6208863_r1
Submitted by: Department of Systems Biology, Columbia University
Study: Isthmus progenitor cells contribute to homeostatic cellular turnover and support regeneration following intestinal injury
show Abstracthide Abstract
The currently accepted intestinal epithelial cell organization model equates crypt base columnar (CBC) cells, marked by high levels of Lgr5 expression, with the intestinal stem cell (ISC). However, recent intestinal regeneration studies have uncovered limitations of the 'Lgr5-CBC' model, leading to two major views: one favoring the presence of a quiescent reserve stem cell population, the other calling for differentiated cell plasticity. To test if an alternative model may help reconcile these perspectives, we studied the hierarchical organization of crypt epithelial cells in an unbiased fashion, by combining high-resolution, single-cell profiling and lineage tracing in multiple transgenic mouse models. These show that Lgr5 is not a specific ISC marker; rather, cells located in the crypt isthmus, which include Lgr5low cells, comprise the ISCs that sustain tissue homeostasis. Following irradiation or intestinal injury, surviving ISCs and progenitors, but not differentiated cells, participate in intestinal regeneration, suggesting that neither de-differentiation nor reserve stem cell populations are drivers of intestinal regeneration. Our results provide a novel viewpoint for the intestinal crypt epithelium, in which ISCs localize to the crypt isthmus, and ISC potential is restricted to stem and progenitor cells. Overall design: Single-cell RNA-Seq data of highly purified mouse intestinal crypt epithelial cells
Sample: Mouse intestinal crypt epithelial cells from adult male C57BL/6J (8 weeks old), untreated, scRNA-seq
SAMN28794764 • SRS13253832 • All experiments • All runs
Organism: Mus musculus
Library:
Name: GSM6208863
Instrument: Illumina NovaSeq 6000
Strategy: RNA-Seq
Source: TRANSCRIPTOMIC SINGLE CELL
Selection: cDNA
Layout: PAIRED
Construction protocol: Library preparation and sequencing were performed by the JP Sulzberger Columbia Genome Centre (Single cell analysis core), using standard methodologies. For scRNA-seq crypt epithelial cells were sorted to exclude dead cells and contaminating villi (Alive/Epcam+/B6A6-). Immediately after sorting, cells were counted using an automated cell counter (ThermoFisher Countess II FL) to check viability and processed for library preparation (10x chromium). For single cell Multiome, immediately after sorting, isolated cells (>100'000) were processed to extract nuclei following manufacturer recommendation (protocol CG000365, Rev B). Isolated nuclei were counted and quality control using an automated cell counter (ThermoFisher Countess II FL) and immediately processed for library preparation. single-cell RNA-seq and snRNA-Seq+snATAC-Seq (multiome)
Runs: 1 run, 413.9M spots, 41.8G bases, 11.2Gb
Run# of Spots# of BasesSizePublished
SRR19489867413,884,63441.8G11.2Gb2024-03-24

ID:
22130478

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