Substrate Specificity of the TRAMP Nuclear Surveillance Complexes

Delan-Forino, Clémentine; Spanos, Christos; Rappsilber, Juri; Tollervey, David

doi:10.1101/2020.03.04.976274

Cited by 4 publications

(7 citation statements)

References 59 publications

(91 reference statements)

Supporting

Mentioning

Contrasting

Order By: Relevance

“…RNA can also be degraded by Rrp6 exonuclease that is located on the top of the exosome. In addition, it has been proposed that RNA can access Dis3 directly without passing through the channel ("direct access", da conformation) (Bonneau et al, 2009;Delan-Forino et al, 2017;Han and van Hoof, 2016;Liu et al, 2014;Makino et al, 2013Makino et al, , 2015. However, the functional contribution of each model as well the mechanisms that direct routing of substrates have remain unexplored.…”

Section: Comparative Ric With Exosome Mutants Reveals Differences In mentioning

confidence: 99%

“…Behaviour of a given protein in the RIC experiment reflects the mean RNA association of this protein in an ensemble of states. It was suggested that in wild-type, the preferred state of the nuclear exosome is the actively channel-threading conformation (Bonneau et al, 2009;Delan-Forino et al, 2017;Schneider et al, 2012). To test this hypothesis, we sought to perturb the system by using defined mutants of the exosome complex.…”

Section: Comparative Ric With Exosome Mutants Reveals Differences In mentioning

confidence: 99%

“…Hence, the positive shift of the Dis3/Rrp43 signature in the comparative RIC experiment is compatible with an increased use of the da route by poly(A)+ RNA in a rrp6Δ mutant ( Figure 7C). So far, the da conformation has only been observed in S. cerevisiae, and was suggested to prefer short structured substrates, such as pre-tRNAs and hypomodified tRNA (Delan-Forino et al, 2017;Han and van Hoof, 2016). However, an S. cerevisiae mutant that is unable to adopt the da conformationand that has no discernible growth phenotype in a wild-type backgroundshows a synthetic growth defect with rrp6Δ (Han and van Hoof, 2016).…”

Section: Comparative Ric With Exosome Mutants Reveals Differences In mentioning

confidence: 99%

“…Adaptation of the da conformation could explain how functional redundancy between Dis3 and Rrp6 is achieved to allow efficient regulation of cellular RNA levels. This would enable Dis3 to execute degradation of Rrp6 substrates in its absence (Delan-Forino et al, 2017).…”

Section: Comparative Ric With Exosome Mutants Reveals Differences In mentioning

confidence: 99%

See 3 more Smart Citations

System-wide analyses of the fission yeast poly(A)+ RNA interactome reveal insights into organisation and function of RNA-protein complexes

Kilchert

Kecman

Priest

et al. 2019

Preprint

View full text Add to dashboard Cite

Abbreviations: gene ontology (GO); messenger RNA (mRNA); mass spectrometry (MS); polyadenylation site (PAS); RNA-binding domain (RBD); RNA-binding protein (RBP);RNA interactome capture (RIC); ribonucleoprotein particle (RNP); ribosomal protein (RP); transcription elongation factor (TEF); wild-type (WT); whole cell extract (WCE); cleavage and polyadenylation factor (CPF); cleavage factors IA and IB (CFIA and CFIB) 2 Abstract Production, function, and turnover of mRNA are orchestrated by multi-subunit machineries that play a central role in gene expression. Within these molecular machines, interactions with the target mRNA are mediated by RNA-binding proteins (RBPs), and the accuracy and dynamics of these RNA-protein interactions are essential for their function. Here, we show that fission yeast whole cell poly(A)+ RNA-protein crosslinking data provides system-wide information on the organisation and function of the RNA-protein complexes. We evaluate relative enrichment of cellular RBPs on poly(A)+ RNA to identify interactors with high RNAbinding activity and provide key information about the RNA-binding properties of large multiprotein complexes, such as the mRNA 3' end processing machinery (cleavage and polyadenylation factor, CPF) and the RNA exosome. We demonstrate that different functional modules within CPF differ in their ability to interact with RNA. Importantly, we reveal that CPF forms additional contacts with RNA via the Fip1 subunit of the polyadenylation module and two subunits of the nuclease module. In addition, our data highlights the central role of the RNA helicase Mtl1 in RNA degradation by the exosome as mutations in Mtl1 lead to disengagement of the exosome from RNA. We examine how routes of substrate access to the complex are affected upon mutation of exosome subunits. Our results provide important insights into how different components of the exosome contribute to engagement of the complex with substrate RNA. Overall, our data uncover how multi-subunit cellular machineries interact with RNA, on a proteome-wide scale.

show abstract

Section: Comparative Ric With Exosome Mutants Reveals Differences In mentioning

confidence: 99%

Section: Comparative Ric With Exosome Mutants Reveals Differences In mentioning

confidence: 99%

Section: Comparative Ric With Exosome Mutants Reveals Differences In mentioning

confidence: 99%

Section: Comparative Ric With Exosome Mutants Reveals Differences In mentioning

confidence: 99%

See 2 more Smart Citations

System-wide analyses of the fission yeast poly(A)+ RNA interactome reveal insights into organisation and function of RNA-protein complexes

Kilchert

Kecman

Priest

et al. 2019

Preprint

View full text Add to dashboard Cite

show abstract

“…Budding yeast TRAMP includes one of two nontemplated poly(A) polymerases of the Polβ family, Trf4 or Trf5, and one of two zinc-knuckle RNA-binding proteins, Air1 or Air2 (24)(25)(26)(27). TRAMP promotes degradation of RNA transcripts produced by all three RNA polymerases (28) through the addition of short oligo-adenylated tails to the 3′ end of RNAs (24,25,29,30).…”

mentioning

confidence: 99%

Substrate discrimination and quality control require each catalytic activity of TRAMP and the nuclear RNA exosome

Das

Zattas

Zinder

et al. 2021

Proc. Natl. Acad. Sci. U.S.A.

View full text Add to dashboard Cite

Quality control requires discrimination between functional and aberrant species to selectively target aberrant substrates for destruction. Nuclear RNA quality control in Saccharomyces cerevisiae includes the TRAMP complex that marks RNA for decay via polyadenylation followed by helicase-dependent 3′ to 5′ degradation by the RNA exosome. Using reconstitution biochemistry, we show that polyadenylation and helicase activities of TRAMP cooperate with processive and distributive exoribonuclease activities of the nuclear RNA exosome to protect stable RNA from degradation while selectively targeting and degrading less stable RNA. Substrate discrimination is lost when the distributive exoribonuclease activity of Rrp6 is inactivated, leading to degradation of stable and unstable RNA species. These data support a proofreading mechanism in which deadenylation by Rrp6 competes with Mtr4-dependent degradation to protect stable RNA while selectively targeting and degrading unstable RNA.

show abstract