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SRX6094327: GSM3897989: Sorted_cells_pool_1; Mus musculus; RNA-Seq
1 ILLUMINA (Illumina HiSeq 4000) run: 450.1M spots, 90G bases, 43Gb downloads

Submitted by: NCBI (GEO)
Study: Intestinal endocrine subtype specification analyzed by Single Cell RNA-Seq in mouse enteroids/mini-guts.
show Abstracthide Abstract
The goal of this experiment is to decipher the mechanism of intestinal endocrine / enteroendocrine subtype specification, that is far from being fully understood. To this end, we used single cell genomics in mouse mini-guts. Enteroendocrine cells are derived from endocrine progenitors expressing the transcription factor Ngn3. We took advantage of the Ngn3+/eYFP mouse model -where endocrine progenitors and their descendants can be isolated and sorted by FACS on the basis of the eYFP fluorescence- and established enteroids or mini-guts from the small intestine. Enteroids were dissociated and eYFP+ single cells were directly sorted in 96 wells of the Precise WTA Single Cell Encoding Plate (BD™ Precise WTA Single Cell Kit, BD Genomics). cDNA and libraries were prepared following the BD protocol. Sequencing (paired-end, 2x100b) was performed in a HiSeq 4000 (Illumina). The bioinformatic analysis allowed to identify 8 different groups of enteroendocrine cells with specific signatures. Overall design: Cells from Ngn3eYFP mice enteroids were sorted and captured. Their transcriptomes were analyzed by single-cell RNASeq.
Sample: Sorted_cells_pool_1
SAMN12095470 • SRS4995309 • All experiments • All runs
Organism: Mus musculus
Library:
Instrument: Illumina HiSeq 4000
Strategy: RNA-Seq
Source: TRANSCRIPTOMIC
Selection: cDNA
Layout: PAIRED
Construction protocol: To dissociate the enteroids, the culture medium was removed and the Matrigel was broken. Then, the enteroids were digested to single cells in 500µL of TrypLE™ Express Enzyme (1X) (Gibco™) at 37°C for 20min. The dissociation was improved by passaging into a syringe mounted with a 18G needle. The digestion was stopped by addition of Advanced DMEM/F-12, fetal calf serum 10%, N-acetylcysteine 0,5mM, B27 1X. The cells were pelleted, washed 2 times and resuspended in the same medium. Finally, they are filtered on a 50 µm cell strainer. eYFP+ cells, from dissociated Neurog3eYFP/+ enteroids, were sorted directly into 96 well plates « Precise WTA Single Cell Encoding Plate » (BD™ Precise WTA Single Cell Kit, BD Genomics) (1 cell/well) using a FACS Aria Fusion (BD). DAPI was used to sort only living cells. Cells were sorted directly into four 96 well plates « Precise WTA Single Cell Encoding Plate » (BDTM Precise WTA Single Cell Kit, BD Genomics) (1 cell/well) using a FACSAria II (BD). The library was prepared by the GenomEast Platform (IGBMC) following the protocol « Library Preparation with the BDTM Precise WTA Single Cell Kit User's Guide » (910000014 Rev. 02 11/2016, BD Genomics).
Experiment attributes:
GEO Accession: GSM3897989
Links:
Runs: 1 run, 450.1M spots, 90G bases, 43Gb
Run# of Spots# of BasesSizePublished
SRR9327493450,083,91590G43Gb2019-08-15

ID:
8148196

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