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Series GSE73926

Query DataSets for GSE73926

Status

Public on Feb 15, 2016

Title

Genome-wide MAF1-dependent regulation of RNA polymerase III transcription [ChIP-Seq]

Organism

Experiment type

Genome binding/occupancy profiling by high throughput sequencing

Summary

In higher eukaryotes, an important mechanism to tune translation in different tissues and conditions is mTORC1-dependent regulation of tRNAs transcription by RNA polymerase III (Pol III), as the relative amount of tRNAs tightly coordinates with the translational needs of the cell. mTORC1 contributes to regulate protein synthesis through its direct substrate MAF1, which functions as a negative regulator of Pol III transcription in response to stimuli such as serum starvation or rapamycin treatment. Here, we applied ChIP-seq to examine the Pol III occupancy profile in human fibroblasts and report evidence of a genome wide, MAF1-dependent coordinated response to favorable or stress growth conditions. Strikingly, while a set of genes is extremely responsive in terms of Pol III binding, other genes are mostly unperturbed, yet associated with transcriptionally engaged polymerases as revealed by nascent EU-labeled RNA-seq (neuRNA-seq). As shown by DamIP-seq, the responsiveness of a subset of genes is tightly connected to the rapid and transient interaction of MAF1 with DNA-bound Pol III.

Overall design

We performed duplicate ChIP-seq experiments for the Rpc4 (POLR3D) subunit of RNA polymerase III in IMR90hTert cells grown in the presence of fetal bovine serum (FBS), serum starved (SS), serum starved and treated with insulin (SS+I), serum starved and treated with insulin and rapamycin (SS+R+I). Additional ChIP-seq profiles were generated in cells treated with MAF1 siRNAs and serum starved. MAF1 binding was addressed by DamIP-seq, using two replicates per clone of IMR90hTert cells expressing HA-tagged MAF1-DamK9A (2 different clones) or EGFP-DamK9A (2 different clones). To monitor dynamic transcription profiles we did neusRNA-seq in IMR90hTert cells EU-labeled or mock (DMSO)-labeled. For both DamIP-seq and neusRNA-seq, cells were either unperturbed or serum starved.

Contributor(s)

Orioli A, Praz V, l'Hote P, Hernandez N

Citation(s)

Submission date

Oct 13, 2015

Last update date

May 15, 2019

Contact name

Nicolo Riggi

Organization name

CHUV

Department

Département de Pathologie Expérimentale

Lab

Institut universitaire de pathologie

Street address

Bugnon 25

City

Lausanne

State/province

VD

ZIP/Postal code

1011

Country

Switzerland

Platforms (1)

Illumina HiSeq 2500 (Homo sapiens)

Samples (22)

More...

GSM1906345	ChIP-seq Rpc4 IMR90hTert cells, (FBS) rep1
GSM1906346	ChIP-seq Rpc4 IMR90hTert cells, (FBS) rep2
GSM1906347	ChIP-seq Rpc4 IMR90hTert cells, (SS) rep1

This SubSeries is part of SuperSeries:

Genome-wide MAF1-dependent regulation of RNA polymerase III transcription

Relations

BioProject

SRA

Download family	Format
SOFT formatted family file(s)	SOFT
MINiML formatted family file(s)	MINiML
Series Matrix File(s)	TXT

Supplementary file	Size	Download	File type/resource
GSE73926_RAW.tar	29.5 Mb	(http)(custom)	TAR (of BEDGRAPH)
SRA Run Selector
Raw data are available in SRA
Processed data provided as supplementary file

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