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SRX22586607: GSM7910915: Alim Diapause 1 Month ATACseq Rep1.5; Austrofundulus limnaeus; ATAC-seq
1 ILLUMINA (NextSeq 550) run: 98.3M spots, 11.8G bases, 5.2Gb downloads

Submitted by: NCBI (GEO)
Study: Comparative ATACseq Between Killifish Species
show Abstracthide Abstract
We evaluate the global chromatin changes that occur during the developmental progression and development-to-diapause transition in a closely related set of killifish species. Overall design: Time-course examination the global chromatin landscape changes during the tranistion from development-to-diapause in the African turquoise killifish, South American killifish, and equivalent developmental stages in the red-striped and lyretail killifish.
Sample: Alim Diapause 1 Month ATACseq Rep1.5
SAMN38334746 • SRS19593540 • All experiments • All runs
Library:
Instrument: NextSeq 550
Strategy: ATAC-seq
Source: GENOMIC
Selection: other
Layout: PAIRED
Construction protocol: To generate nuclei-suspension for ATAC-seq libraries, snap frozen embryo samples (~10 embryos per sample) were thawed for 1 minute and resuspended at 4oC in 200ml EZ-lysis buffer (Sigma Aldritch No. 3408). Samples were then transferred to 250 ml mini-douncers (DWK (Kimble) 885300-0000) and dounced 25 times with pestle A and B respectively. After a 2 minute incubation following douncing, samples were spun at 500g for 5 minutes to precipitate nuclei, and the EZ-lysis supernatant was removed. Nuclei were then resuspended in 250ml PBS (ThermoFisher No. AM9624) and an aliquot of 5µl of nuclei was incubated with 5ml of 0.4% trypan blue stain (ThermoFisher No. 15250061) for counting the total intact nuclei counts. Samples of ~25,000 nuclei were then suspended in a Tn5 transposition mix (65ml of tagmentation DNA buffer (Illumina No. 20034197), 63ml of nuclease-free water, and 2.5ml of tagmentation DNA enzyme I (e.g Tn5 transposase) (Illumina No. 20034197) for 20 minutes at 37oC. Following incubation, the mix was purified using the Qiagen mini-elute kit (Qiagen No. 28206) to isolate tagmented DNA. PCR amplification and subsequent qPCR monitoring was performed as described in the original ATAC-seq protocol (~14-18 cycles of PCR). Amplified DNA from the PCR reaction was purified using the Qiagen mini-elute kit (Qiagen No. 28206), as recommended by the manufacturer. Samples were subsequently pooled and sequenced using next-generation short-read sequencing on an Illumina NEXTseq 550.
Experiment attributes:
GEO Accession: GSM7910915
Links:
Runs: 1 run, 98.3M spots, 11.8G bases, 5.2Gb
Run# of Spots# of BasesSizePublished
SRR2689233098,307,26311.8G5.2Gb2024-06-18

ID:
30586459

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