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Links from GEO DataSets

Items: 5

1.

Comparison of endogenous tRNA expression levels from cells expressing and sgRNA from either a U6 or tRNA promoter

(Submitter supplied) The goal of this study was to compare the endogenous tRNA expression levels from cells transduced with a lentiviral vector encopding Cas9 and an sgRNA from a U6 or a Glutamine tRNA promoter. Using high-throughput sequencing methods (Illumina Hi-Seq 2000) we show that endogenous tRNA expression levels are not perturbed by expression of an sgRNA from a human tRNA.
Organism:
Homo sapiens
Type:
Non-coding RNA profiling by high throughput sequencing
Platform:
GPL11154
3 Samples
Download data: TXT
Series
Accession:
GSE69720
ID:
200069720
2.

A viral guide RNA delivery system for CRISPR-based transcriptional activation and heritable targeted DNA demethylation

(Submitter supplied) CRISPR-based epigenome editing was recently used to activate gene expression through direct transcriptional activation or site-specific DNA demethylation. Viral delivery of guide RNAs for these purposes remains to be developed. Furthermore, currently available viral delivery tools for genome editing show meager rates of heritability. Here, we have developed a tobacco rattle virus (TRV)-based guide RNA delivery system for both transcriptional activation and targeted DNA demethylation. more...
Organism:
Arabidopsis thaliana
Type:
Methylation profiling by high throughput sequencing
Platforms:
GPL17639 GPL26208
12 Samples
Download data: BED, BW, TXT
Series
Accession:
GSE148934
ID:
200148934
3.

Engineered miniature CRISPR-Cas system for mammalian genome regulation and editing

(Submitter supplied) Compact and versatile CRISPR-Cas systems will enable genome engineering applications through high-efficiency delivery in a wide variety of contexts. Here we create an efficient miniature Cas system (CasMINI) engineered from the type V-F Cas12f (Cas14) system by guide RNA and protein engineering, which is less than half the size of currently used CRISPR systems (Cas9 or Cas12a). We demonstrate that CasMINI can drive high levels of gene activation (up to thousands-fold increases), while the natural Cas12f system fails to function in mammalian cells. more...
Organism:
Homo sapiens
Type:
Expression profiling by high throughput sequencing
Platform:
GPL24676
8 Samples
Download data: TAB
Series
Accession:
GSE180773
ID:
200180773
4.

Expression data from human 293 cells

(Submitter supplied) A long form (tRNase ZL) of tRNA 3' processing endoribonuclease (tRNase Z, or 3' tRNase) can cleave any target RNA at any desired site under the direction of artificial small guide RNA (sgRNA). We discovered in human kidney 293 cell extracts various new small noncoding RNAs (ncRNAs) including 5'-half-tRNAs and 28S rRNA fragments, co-immunoprecipitated with tRNase ZL, and demonstrated that two of these ncRNAs work as sgRNAs for tRNase ZL in vivo as well as in vitro. more...
Organism:
Homo sapiens
Type:
Expression profiling by array
Platform:
GPL570
2 Samples
Download data: CEL, CHP
Series
Accession:
GSE12524
ID:
200012524
5.

LADL: Light-activated dynamic looping for endogenous gene expression control

(Submitter supplied) Mammalian genomes are folded into tens of thousands of long-range looping interactions1,2. The cause and effect relationship between looping and genome function is poorly understood, and the extent to which chromatin loops are dynamic on short time scales remains a fundamental unanswered question. Currently available strategies for loop engineering involve synthetic transcription factors tethered to dCas93,4or zinc fingers5,6, which are constitutively expressed5,6or induced on long time scales by the presence of a small molecule3.Here we report a new class of 3D optoepigenetic toolsfor the directed rearrangement of 3D chromatin looping on short time scales using blue light. more...
Organism:
Mus musculus
Type:
Other
Platform:
GPL19057
20 Samples
Download data: BED, TXT
Series
Accession:
GSE115963
ID:
200115963
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