RNA Polymerase II CTD phosphatase Rtr1 fine-tunes transcription termination

Victorino, José; Fox, Melanie J.; Smith-Kinnaman, Whitney R.; Justice, Sarah A. Peck; Burriss, Katlyn Hughes; Boyd, Asha K.; Zimmerly, Megan A.; Chan, Rachel R.; Hunter, Gerald O.; Liu, Yunlong; Mosley, Amber L.

doi:10.1371/journal.pgen.1008317

Cited by 16 publications

(35 citation statements)

References 114 publications

(199 reference statements)

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“…Rtr1 ("regulator of transcription" 1) has been described as a phosphorylated RNA pol II interactor by acting as an S5-P CTD phosphatase during the transition from the initiation of the transcription to elongation in vivo (Gibney et al, 2008;Mosley et al, 2009Mosley et al, , 2013Hsu et al, 2014;Smith-Kinnaman et al, 2014;Hunter et al, 2016). Additional roles have been proposed for Rtr1 in transcription and mRNA stability (Mosley et al, 2013;Hsu et al, 2014;Hodko et al, 2016;Victorino et al, 2020) (our unpublished data).…”

Section: Rtr1/rpap2mentioning

confidence: 82%

Biogenesis of RNA Polymerases in Yeast

Garrido-Godino

Gutiérrez-Santiago

Navarro

2021

Front. Mol. Biosci.

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Eukaryotic RNA polymerases (RNA pols) transcriptional processes have been extensively investigated, and the structural analysis of eukaryotic RNA pols has been explored. However, the global assembly and biogenesis of these heteromultimeric complexes have been narrowly studied. Despite nuclear transcription being carried out by three RNA polymerases in eukaryotes (five in plants) with specificity in the synthesis of different RNA types, the biogenesis process has been proposed to be similar, at least for RNA pol II, to that of bacteria, which contains only one RNA pol. The formation of three different interacting subassembly complexes to conform the complete enzyme in the cytoplasm, prior to its nuclear import, has been assumed. In Saccharomyces cerevisiae, recent studies have examined in depth the biogenesis of RNA polymerases by characterizing some elements involved in the assembly of these multisubunit complexes, some of which are conserved in humans. This study reviews the latest studies governing the mechanisms and proteins described as being involved in the biogenesis of RNA polymerases in yeast.

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Section: Rtr1/rpap2mentioning

confidence: 82%

Biogenesis of RNA Polymerases in Yeast

Garrido-Godino

Gutiérrez-Santiago

Navarro

2021

Front. Mol. Biosci.

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“…Previously performed experiments found that the entire CPF complex copurifies with FLAG-tagged Pta1 35 . In theory, addition of an affinity purified CPF sample to one channel of the TMT multiplex would increase the MS1 ion intensity of CPF subunits and would “trigger” the mass spectrometer to pick peptides from CPF complex subunits more often in a DDA analysis than in samples that lack an isobaric trigger.…”

Section: Resultsmentioning

confidence: 99%

“…To boost detection of the native CPF subunits, subsequent mTPP replicates of WT and ssu72-2 included the addition of a trigger channel consisting of an affinity-purified CPF complexes. Affinity purification of CPF via Pta1-FLAG was performed as described previously for Ssu72-FLAG purifications 35 . The Pta1-FLAG affinity purified sample was added at a ratio of 6.25 ug trigger to 50 ug of the lowest heat-treated sample (1:8 ratio) for the initial study.…”

Section: Methodsmentioning

confidence: 99%

“…As a proof-of-concept, we investigated the ability of this approach to enhance detection of the relatively low abundance protein complex cleavage and polyadenylation factor (CPF) complex in a mTPP workflow. Affinity purified CPF that we have previously characterized [35][36][37][38][39] was incorporated as an isobaric trigger channel into our mTPP workflow at a ratio to the lowest heat-treated mTPP sample of ~1:8 and ~1:50. Using this approach, a significant increase in the abundance of CPF complex members was observed, including those that were not readily identified without the isobaric trigger channel.…”

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confidence: 99%

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Boosting detection of low abundance proteins in thermal proteome profiling experiments by addition of an isobaric trigger channel to TMT multiplexes

Justice

McCracken

Victorino

et al. 2020

Preprint

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The study of low abundance proteins is a challenge to discovery-based proteomics. Mass-spectrometry (MS) applications, such as thermal proteome profiling (TPP) face specific challenges in detection of the whole proteome as a consequence of the use of nondenaturing extraction buffers. TPP is a powerful method for the study of protein thermal stability, but quantitative accuracy is highly dependent on consistent detection. Therefore, TPP can be limited in its amenability to study low abundance proteins that tend to have stochastic or poor detection by MS. To address this challenge, we incorporated an affinity purified protein complex sample at submolar concentrations as an isobaric trigger channel into a mutant TPP (mTPP) workflow to provide reproducible detection and quantitation of the low abundance subunits of the Cleavage and Polyadenylation Factor (CPF) complex. The inclusion of an isobaric protein complex trigger channel increased detection an average of 40x for previously detected subunits and facilitated detection of CPF subunits that were previously below the limit of detection. Importantly, these gains in CPF detection did not cause large changes in melt temperature (Tm) calculations for other unrelated proteins in the samples, with a high positive correlation between Tm estimates in samples with and without isobaric trigger channel addition. Overall, the incorporation of affinity purified protein complex as an isobaric trigger channel within a TMT multiplex for mTPP experiments is an effective and reproducible way to gather thermal profiling data on proteins that are not readily detected using the original TPP or mTPP protocols.

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“…Affinity purification of native CPF via Pta1-FLAG was performed as described previously for Ssu72-FLAG purifications. 37 The Pta1-FLAG affinity-purified sample was added at a ratio of 6.25 μg trigger to 50 μg of the lowest heat-treated sample (1:8 ratio) for the biological replicates. The untreated samples were removed from the multiplex from no trigger samples to accommodate for the isobaric trigger channel to be labeled with TMT126.…”

Section: Experimental Sectionmentioning

confidence: 99%

Boosting Detection of Low-Abundance Proteins in Thermal Proteome Profiling Experiments by Addition of an Isobaric Trigger Channel to TMT Multiplexes

et al. 2021

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The study of low-abundance proteins is a challenge to discovery-based proteomics. Mass spectrometry (MS) applications, such as thermal proteome profiling (TPP), face specific challenges in the detection of the whole proteome as a consequence of the use of nondenaturing extraction buffers. TPP is a powerful method for the study of protein thermal stability, but quantitative accuracy is highly dependent on consistent detection. Therefore, TPP can be limited in its amenability to study low-abundance proteins that tend to have stochastic or poor detection by MS. To address this challenge, we incorporated an affinity-purified protein complex sample at submolar concentrations as an isobaric trigger channel into a mutant TPP (mTPP) workflow to provide reproducible detection and quantitation of the low-abundance subunits of the cleavage and polyadenylation factor (CPF) complex. The inclusion of an isobaric protein complex trigger channel increased detection an average of 40× for previously detected subunits and facilitated detection of CPF subunits that were previously below the limit of detection. Importantly, these gains in CPF detection did not cause large changes in melt temperature ( T m ) calculations for other unrelated proteins in the samples, with a high positive correlation between T m estimates in samples with and without isobaric trigger channel addition. Overall, the incorporation of an affinity-purified protein complex as an isobaric trigger channel within a tandem mass tag (TMT) multiplex for mTPP experiments is an effective and reproducible way to gather thermal profiling data on proteins that are not readily detected using the original TPP or mTPP protocols.

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RNA Polymerase II CTD phosphatase Rtr1 fine-tunes transcription termination

Cited by 16 publications

References 114 publications

Biogenesis of RNA Polymerases in Yeast

Biogenesis of RNA Polymerases in Yeast

Boosting detection of low abundance proteins in thermal proteome profiling experiments by addition of an isobaric trigger channel to TMT multiplexes

Boosting Detection of Low-Abundance Proteins in Thermal Proteome Profiling Experiments by Addition of an Isobaric Trigger Channel to TMT Multiplexes

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