Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Pivot Concepts:
Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Target Concepts:
Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Query: EC:2.7.7.6 (
RNA polymerase
)
34,946
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
Many cancer-causing chromosomal translocations result in transactivating protein products encoding FET family (
FUS
, EWSR1, TAF15) low-complexity (LC) domains fused to a DNA binding domain from one of several transcription factors. Recent work demonstrates that higher-order assemblies of FET LC domains bind the carboxy-terminal domain of the large subunit of
RNA polymerase II
(RNA pol II CTD), suggesting FET oncoproteins may mediate aberrant transcriptional activation by recruiting
RNA polymerase II
to promoters of target genes. Here we use nuclear magnetic resonance (NMR) spectroscopy and hydrogel fluorescence microscopy localization and fluorescence recovery after photobleaching to visualize atomic details of a model of this process, interactions of RNA pol II CTD with high-molecular weight TAF15 LC assemblies. We report NMR resonance assignments of the intact degenerate repeat half of human RNA pol II CTD alone and verify its predominant intrinsic disorder by molecular simulation. By measuring NMR spin relaxation and dark-state exchange saturation transfer, we characterize the interaction of RNA pol II CTD with amyloid-like hydrogel fibrils of TAF15 and hnRNP A2 LC domains and observe that heptads far from the acidic C-terminal tail of RNA pol II CTD bind TAF15 fibrils most avidly. Mutation of CTD lysines in heptad position 7 to consensus serines reduced the overall level of TAF15 fibril binding, suggesting that electrostatic interactions contribute to complex formation. Conversely, mutations of position 7 asparagine residues and truncation of the acidic tail had little effect. Thus, weak, multivalent interactions between TAF15 fibrils and heptads throughout RNA pol II CTD collectively mediate complex formation.
...
PMID:Lysines in the RNA Polymerase II C-Terminal Domain Contribute to TAF15 Fibril Recruitment. 2894 58
Mutations in multiple RNA/DNA binding proteins cause Amyotrophic Lateral Sclerosis (ALS). Included among these are the three members of the FET family (
FUS
, EWSR1 and TAF15) and the structurally similar MATR3. Here, we characterized the interactomes of these four proteins, revealing that they largely have unique interactors, but share in common an association with U1 snRNP. The latter observation led us to analyze the interactome of the U1 snRNP machinery. Surprisingly, this analysis revealed the interactome contains ~220 components, and of these, >200 are shared with the
RNA polymerase II
(RNAP II) machinery. Among the shared components are multiple ALS and Spinal muscular Atrophy (SMA)-causative proteins and numerous discrete complexes, including the SMN complex, transcription factor complexes, and RNA processing complexes. Together, our data indicate that the RNAP II/U1 snRNP machinery functions in a wide variety of molecular pathways, and these pathways are candidates for playing roles in ALS/SMA pathogenesis.
...
PMID:Interactome analyses revealed that the U1 snRNP machinery overlaps extensively with the RNAP II machinery and contains multiple ALS/SMA-causative proteins. 2988 7
FUS
(fused in sarcoma) plays a key role in several steps of RNA metabolism, and dominant mutations in this protein are associated with neurodegenerative diseases. Here, we show that
FUS
is a component of the cellular response to topoisomerase I (TOP1)-induced DNA breakage; relocalising to the nucleolus in response to
RNA polymerase II
(Pol II) stalling at sites of TOP1-induced DNA breaks. This relocalisation is rapid and dynamic, reversing following the removal of TOP1-induced breaks and coinciding with the recovery of global transcription. Importantly,
FUS
relocalisation following TOP1-induced DNA breakage is associated with increased
FUS
binding at sites of
RNA polymerase I
transcription in ribosomal DNA and reduced
FUS
binding at sites of RNA Pol II transcription, suggesting that
FUS
relocates from sites of stalled RNA Pol II either to regulate pre-mRNA processing during transcriptional stress or to modulate ribosomal RNA biogenesis. Importantly,
FUS
-mutant patient fibroblasts are hypersensitive to TOP1-induced DNA breakage, highlighting the possible relevance of these findings to neurodegeneration.
...
PMID:FUS (fused in sarcoma) is a component of the cellular response to topoisomerase I-induced DNA breakage and transcriptional stress. 3080 50
pncRNA-D
is an irradiation-induced 602-nt long noncoding RNA transcribed from the promoter region of the cyclin D1 (
CCND1
) gene.
CCND1
expression is predicted to be inhibited through an interplay between
pncRNA-D
and RNA-binding protein TLS/
FUS
. Because the
pncRNA-D
-TLS interaction is essential for
pncRNA-D
-stimulated
CCND1
inhibition, here we studied the possible role of RNA modification in this interaction in HeLa cells. We found that osmotic stress induces
pncRNA-D
by recruiting
RNA polymerase II
to its promoter.
pncRNA-D
was highly m
6
A-methylated in control cells, but osmotic stress reduced the methylation and also arginine methylation of TLS in the nucleus. Knockdown of the m
6
A modification enzyme methyltransferase-like 3 (METTL3) prolonged the half-life of
pncRNA-D
, and among the known m
6
A recognition proteins, YTH domain-containing 1 (YTHDC1) was responsible for binding m
6
A of
pncRNA-D
Knockdown of METTL3 or YTHDC1 also enhanced the interaction of
pncRNA-D
with TLS, and results from RNA pulldown assays implicated YTHDC1 in the inhibitory effect on the TLS-
pncRNA-D
interaction. CRISPR/Cas9-mediated deletion of candidate m
6
A site decreased the m
6
A level in
pncRNA-D
and altered its interaction with the RNA-binding proteins. Of note, a reduction in the m
6
A modification arrested the cell cycle at the G
0
/G
1
phase, and
pncRNA-D
knockdown partially reversed this arrest. Moreover,
pncRNA-D
induction in HeLa cells significantly suppressed cell growth. Collectively, these findings suggest that m
6
A modification of the long noncoding RNA
pncRNA-D
plays a role in the regulation of
CCND1
gene expression and cell cycle progression.
...
PMID:Long noncoding RNA
pncRNA-D
reduces cyclin D1 gene expression and arrests cell cycle through RNA m
6
A modification. 3216 96
RNA processing occurs co-transcriptionally through the dynamic recruitment of RNA processing factors to
RNA polymerase II
(RNAPII). However, transcriptome-wide identification of protein-RNA interactions specifically assembled on transcribing RNAPII is challenging. Here, we develop the targeted RNA immunoprecipitation sequencing (tRIP-seq) method that detects protein-RNA interaction sites in thousands of cells. The high sensitivity of tRIP-seq enables identification of protein-RNA interactions at functional subcellular levels. Application of tRIP-seq to the
FUS
-RNA complex in the RNAPII machinery reveals that
FUS
binds upstream of alternative polyadenylation (APA) sites of nascent RNA bound to RNAPII, which retards RNAPII and suppresses the recognition of the polyadenylation signal by CPSF. Further tRIP-seq analyses demonstrate that the repression of APA is achieved by a complex composed of
FUS
and U1 snRNP on RNAPII, but not by either one alone. Moreover, our analysis reveals that
FUS
mutations in familial amyotrophic lateral sclerosis (ALS) that impair the
FUS
-U1 snRNP interaction aberrantly activate the APA sites. tRIP-seq provides new insights into the regulatory mechanism of co-transcriptional RNA processing by RNA processing factors.
...
PMID:tRIP-seq reveals repression of premature polyadenylation by co-transcriptional FUS-U1 snRNP assembly. 3218 59
<< Previous
1
2
3
