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DRX571524: NextSeq 1000 paired end sequencing of SAMD00813918
1 ILLUMINA (NextSeq 1000) run: 47.6M spots, 4.8G bases, 2.3Gb downloads

Submitted by: Tokyo Metropolitan Institute of Medical Science
Study: RNA-DNA hybrids on protein coding genes are stabilized by loss of RNase H and are associated with DNA damages during S-phase in fission yeast
show Abstracthide Abstract
RNA-DNA hybrid is a part of the R-loop which is an important non-standard nucleic acid structure. RNA-DNA hybrid-R-loop causes genomic instability by inducing DNA damages or inhibiting DNA replication. It also plays biologically important roles in regulation of transcription, replication, recombination and repair. Here, we have employed catalytically inactive human RNase H1 mutant (D145N) to visualize RNA-DNA hybrids and map their genomic locations in fission yeast cells. The RNA-DNA hybrids appear as multiple nuclear foci in rnh1rnh201 mutant cells lacking cellular RNase H activity, but not in the wild-type. The majority of RNA-DNA hybrid loci are detected at the protein coding regions and tRNA. In rnh1rnh201 mutant cells, cells with multiple Rad52 foci increase during S-phase and about 20% of the RNA-DNA hybrids overlap with Rad52 loci. During S-phase, more robust association of Rad52 with RNA-DNA hybrids was observed in the protein coding region than in M-phase. These results suggest that persistent RNA-DNA hybrids in the protein coding region in rnh1rnh201 mutant cells generate DNA damages during S-phase, potentially through collision with DNA replication forks.
Sample: H1DH2D_RNaseH1(D145N)_3FLAG_Input
SAMD00813918 • DRS402532 • All experiments • All runs
Library:
Name: 13_H1DH2D_RNaseH1(D145N)_3FLAG_Input
Instrument: NextSeq 1000
Strategy: ChIP-Seq
Source: GENOMIC
Selection: ChIP
Layout: PAIRED
Construction protocol: NEBNext Ultra II DNA Library Prep Kit for Illumina
Runs: 1 run, 47.6M spots, 4.8G bases, 2.3Gb
Run# of Spots# of BasesSizePublished
DRR59097747,579,9344.8G2.3Gb2024-08-27

ID:
34899841

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