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SRX14424035: GSM5943595: cs_bisulfite_spikelet_I; Triticum aestivum; Bisulfite-Seq
2 ILLUMINA (HiSeq X Ten) runs: 645.5M spots, 193.7G bases, 60.5Gb downloads

External Id: GSM5943595_r1
Submitted by: Functional Epigenomics Group, National Key Laboratory of Plant Molecular Genetics, Institute of Plant Physiology and Ecology,Chinese Academy of Sciences
Study: Subgenome-specific usage of transposable element-derived promoters and enhancers in bread wheat development
show Abstracthide Abstract
Transcription start site (TSS) is the hub integrating regulatory input from promoters and enhancers. Common wheat converged three subgenomes adapted to different environment and established as a major crop worldwide. Detection of more precise and new TSS of both genes and enhancers in common wheat is the basis in interpreting transcriptional regulatory networks as well as the subgenome divergent regulation in their entirety. Overall design: In the present study, we profiled the genome wide TSS by CAGE-seq together with DNA methylation and histone modifications from four typical tissues in common wheat, the resulting catalogue of enhancers enabled more precise detection of ubiquitous and tissue specific TSS usage of coding genes and enhancers.
Sample: cs_bisulfite_spikelet_I
SAMN26549887 • SRS12233069 • All experiments • All runs
Library:
Name: GSM5943595
Instrument: HiSeq X Ten
Strategy: Bisulfite-Seq
Source: GENOMIC
Selection: RANDOM
Layout: PAIRED
Construction protocol: The seedlings (above-ground parts) in soil were harvested after 9-day growth. The root in Hoagland solution were harvested after 9-day growth. The spikelets at booting stage (Feeke 10) were harvested. The fresh immature embryos (14days post anthesis) were isolated and either frozen in liquid nitrogen For CAGE-seq,total RNA was treated with RQ1 DNase to remove DNA. The total RNA was treated with T4 polynucleotide kinase subsequently digested with Terminator 5´-Phosphate-Dependent Exonuclease to enrich the capped mRNA. Next, reverse transcription was performed with RT primer harboring a 3'-adaptor sequence and randomized hexamer. Subsequently, the 5'adaptor harboring three additional rG at the 3'terminus was added to the RT reaction to allow template switching and tagging of the 5' adaptor. The cDNAs were treated with Exonuclease I to digest the primers, purified and amplified with PCR primers. The libraries were applied to Illumina Novaseq 6000 system for 150 nt paired-end sequencing.
Runs: 2 runs, 645.5M spots, 193.7G bases, 60.5Gb
Run# of Spots# of BasesSizePublished
SRR18286240324,877,93797.5G30.5Gb2023-10-12
SRR18286241320,643,02296.2G30Gb2023-10-12

ID:
20512509

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