The C-terminal domain of the largest subunit of RNA polymerase II interacts with a novel set of serine/arginine-rich proteins.

Yuryev, Anton; Patturajan, Meera; Litingtung, Ying; Joshi, Ravi V.; Gentile, Cristl; Gebara, Maha M.; Corden, Jeffry L.

doi:10.1073/pnas.93.14.6975

Cited by 318 publications

(290 citation statements)

References 46 publications

Supporting

Mentioning

274

Contrasting

Unclassified

Order By: Relevance

“…Nrd1 contains a CID (Meinhart and Cramer 2004;Meinhart et al 2005) that interacts with CTD phosphorylated at Ser5 (Conrad et al 2000;Gudipati et al 2008;Vasiljeva et al 2008a). Nrd1 also interacts with another essential RNA-binding protein, Nab3 (Yuryev et al 1996). Nrd1, Nab3, and Sen1 form the Nrd1 complex, which is detected by ChIP at snoRNAs genes (Kim et al 2006) as well as some mRNAs genes, mainly at promoter regions (Nedea et al 2003).…”

Section: The Nrd1 Complexmentioning

confidence: 99%

“…ChIP analysis showed RNAPII read-through at most snoRNAs genes in a SEN1 mutant strain or a strain defective for its helicase activity (Kim et al 2006;Steinmetz et al 2006b). Sen1 associates with the CTD and also coprecipitates with several snoRNAs and some snRNAs (Yuryev et al 1996;Ursic et al 1997Ursic et al , 2004. Nedea et al (2008) showed that Glc7, the yeast PP1 (protein phophatase-1) catalytic subunit, is also a regulator of snoRNA termination, interacting directly with Sen1.…”

Section: The Nrd1 Complexmentioning

confidence: 99%

See 1 more Smart Citation

Transcription termination by nuclear RNA polymerases

Richard

Manley²

2009

Genes Dev.

286

326

View full text Add to dashboard Cite

Gene transcription in the cell nucleus is a complex and highly regulated process. Transcription in eukaryotes requires three distinct RNA polymerases, each of which employs its own mechanisms for initiation, elongation, and termination. Termination mechanisms vary considerably, ranging from relatively simple to exceptionally complex. In this review, we describe the present state of knowledge on how each of the three RNA polymerases terminates and how mechanisms are conserved, or vary, from yeast to human.

show abstract

Section: The Nrd1 Complexmentioning

confidence: 99%

Section: The Nrd1 Complexmentioning

confidence: 99%

Transcription termination by nuclear RNA polymerases

Richard

Manley²

2009

Genes Dev.

286

326

View full text Add to dashboard Cite

show abstract

“…Band`a' represents Hsp73, which may signify an artifact of our system as the ER domain interacts with the very closely related Hsp70 protein (Smith and Toft, 1993). Band`b' includes a clone for an RNA polymerase II-binding protein (Yuryev et al, 1996) and a clone for subunit of RNA polymerase III (Sepehri and Hernandez, 1997), both of which potentially regulate cell proliferation. Another clone isolated from band`b' encodes fau, an arsenateresistance protein which is also a tumor suppressor (Rossman and Wang, 1999).…”

Section: Inhibition Of Cbf Decreases Cdk4 Levelsmentioning

confidence: 99%

Exogenous cdk4 overcomes reducedcdk4 RNA and inhibition of G1 progression in hematopoietic cells expressing a dominant-negative CBF – a model for overcoming inhibition of proliferation by CBF oncoproteins

Lou¹,

Cao²,

Bernardin³

et al. 2000

Oncogene

View full text Add to dashboard Cite

Core Binding Factor (CBF) is required for the development of de®nitive hematopoiesis, and the CBF oncoproteins AML1-ETO, TEL-AML1, and CBFb-SMMHC are commonly expressed in subsets of acute leukemia. CBFb-SMMHC slows the G1 to S cell cycle transition in hematopoietic cells, but the mechanism of this e ect is uncertain. We have sought to determine whether inhibition of CBF-mediated trans-activation is su cient to slow proliferation. We demonstrate that activation of KRAB-AML1-ER, a protein containing the AML1 DNA-binding domain, the KRAB repression domain, and the Estrogen receptor ligand binding domain, also slows G1, if its DNA-binding domain is intact. Also, exogenous AML1 overcame CBFb-SMMHC-induced inhibition of proliferation. Representational di erence analysis (RDA) identi®ed cdk4 RNA expression as an early target of KRAB-AML1 activation. Inhibition of CBF activities by KRAB-AML1-ER or CBFb-SMMHC rapidly reduced endogenous cdk4 mRNA levels, even in cells proliferating at or near control rates as a result of exogenous cdk4 expression. Over-expression of cdk4, especially a variant which cannot bind p16 INK4a , overcame cell cycle inhibition resulting from activation of KRAB-AML1-ER, although cdk4 did not accelerate proliferation when expressed alone. These ®ndings indicate that mutations which alter the expression of G1 regulatory proteins can overcome inhibition of proliferation by CBF oncoproteins.

show abstract

“…These early genomic efforts suggested that, similar to DNA binding proteins, functional groupings of genes are being bound by RNA binding proteins perhaps as post-transcriptional operons (Keene and Tenenbaum 2002). However, it is not known at which stage of RNA processing these operons are established.Much of pre-mRNA processing is coupled to transcription both physically and functionally, potentially through interactions with the C-terminal domain (CTD) of RNA polymerase II (RNA Pol II) (Mortillaro et al 1996;Yuryev et al 1996;Kim et al 1997). The CTD is phosphorylated as transcription begins.…”

mentioning

confidence: 99%

Genomic localization of RNA binding proteins reveals links between pre-mRNA processing and transcription

Swinburne

Meyer²,

Liu³

et al. 2006

Genome Res.

View full text Add to dashboard Cite

Pre-mRNA processing often occurs in coordination with transcription thereby coupling these two key regulatory events. As such, many proteins involved in mRNA processing associate with the transcriptional machinery and are in proximity to DNA. This proximity allows for the mapping of the genomic associations of RNA binding proteins by chromatin immunoprecipitation (ChIP) as a way of determining their sites of action on the encoded mRNA. Here, we used ChIP combined with high-density microarrays to localize on the human genome three functionally distinct RNA binding proteins: the splicing factor polypyrimidine tract binding protein (PTBP1/hnRNP I), the mRNA export factor THO complex subunit 4 (ALY/THOC4), and the 3Ј end cleavage stimulation factor 64 kDa (CSTF2). We observed interactions at promoters, internal exons, and 3Ј ends of active genes. PTBP1 had biases toward promoters and often coincided with RNA polymerase II (RNA Pol II). The 3Ј processing factor, CSTF2, had biases toward 3Ј ends but was also observed at promoters. The mRNA processing and export factor, ALY, mapped to some exons but predominantly localized to introns and did not coincide with RNA Pol II. Because the RNA binding proteins did not consistently coincide with RNA Pol II, the data support a processing mechanism driven by reorganization of transcription complexes as opposed to a scanning mechanism. In sum, we present the mapping in mammalian cells of RNA binding proteins across a portion of the genome that provides insight into the transcriptional assembly of RNA-protein complexes.[Supplemental material is available online at www.genome.org and http://silver.med.harvard.edu/brodsky/.] RNA binding proteins regulate many stages of RNA metabolism to help determine gene expression programs (for reviews, see Keene and Tenenbaum 2002;Hieronymus and Silver 2004). To prepare mRNA for export to and translation in the cytoplasm, many events including splicing, cleavage of the 3Ј end, and editing occur cotranscriptionally (Kornblihtt et al. 2004;Aguilera 2005a). After transcription, the mRNA-protein complex may reorganize as it is exported to the cytoplasm and prepared for translation (Fairman et al. 2004). Thus, significant efforts have been made to determine how RNA binding proteins interact at genes and/or mRNAs at various stages of mRNA metabolism (Tenenbaum et al. 2000;Brown et al. 2001;Hieronymus and Silver 2003;Ule et al. 2003;Yu et al. 2004). These early genomic efforts suggested that, similar to DNA binding proteins, functional groupings of genes are being bound by RNA binding proteins perhaps as post-transcriptional operons (Keene and Tenenbaum 2002). However, it is not known at which stage of RNA processing these operons are established.Much of pre-mRNA processing is coupled to transcription both physically and functionally, potentially through interactions with the C-terminal domain (CTD) of RNA polymerase II (RNA Pol II) (Mortillaro et al. 1996;Yuryev et al. 1996;Kim et al. 1997). The CTD is phosphorylated as transcription begins. Following...

show abstract

The C-terminal domain of the largest subunit of RNA polymerase II interacts with a novel set of serine/arginine-rich proteins.

Cited by 318 publications

References 46 publications

Transcription termination by nuclear RNA polymerases

Transcription termination by nuclear RNA polymerases

Exogenous cdk4 overcomes reducedcdk4 RNA and inhibition of G1 progression in hematopoietic cells expressing a dominant-negative CBF – a model for overcoming inhibition of proliferation by CBF oncoproteins

Genomic localization of RNA binding proteins reveals links between pre-mRNA processing and transcription

Contact Info

Product

Resources

About