High-throughput sequencing of partially edited trypanosome mRNAs reveals barriers to editing progression and evidence for alternative editing

Simpson, Rachel M.; Bruno, Andrew E.; Bard, Jonathan; Buck, Michael; Read, Laurie K.

doi:10.1261/rna.055160.115

Cited by 42 publications

(155 citation statements)

References 77 publications

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“…To more precisely define the step of editing that is impacted by MRB7260, we next examined the effects of MRB7260 depletion on RNA editing at the sequence population level. We used our previously described protocol that defines the regions in which the 3 ′ to 5 ′ progression of editing is paused upon depletion of essential editing factors (see Supplemental Methods; Simpson et al 2016Simpson et al , 2017. Using this method, a library of pre-edited, partially edited, and fully edited sequences was obtained from two MRB7260 RNAi-induced cDNA samples and 10 uninduced control samples, two from this study and 8 from a previous study (Simpson et al 2017).…”

Section: Effects Of Mrb7260 On Rna Editing At the Sequence Levelmentioning

confidence: 99%

“…Using this method, a library of pre-edited, partially edited, and fully edited sequences was obtained from two MRB7260 RNAi-induced cDNA samples and 10 uninduced control samples, two from this study and 8 from a previous study (Simpson et al 2017). This library was aligned using TREAT (Simpson et al 2016(Simpson et al , 2017. TREAT defines any space between two non-T nucleotides in the cDNA as an editing site (ES), and ESs are numbered from 3 ′ to 5 ′ , the direction in which overall editing progresses (Fig.…”

Section: Effects Of Mrb7260 On Rna Editing At the Sequence Levelmentioning

confidence: 99%

“…2B). An editing stop site is defined by TREAT as the 5 ′ -most ES that matches the fully edited sequence, and thus any ES 3 ′ of an editing stop site matches the canonical fully edited sequence while the region 5 ′ of the editing stop site contains either pre-edited or junction sequence (Simpson et al 2016). Junctions are variable edited sequences that match neither pre-edited nor fully edited sequence, and are present in partially edited mRNAs between the 3 ′ fully edited and 5 ′ pre-edited regions.…”

Section: Effects Of Mrb7260 On Rna Editing At the Sequence Levelmentioning

confidence: 99%

“…Junctions are variable edited sequences that match neither pre-edited nor fully edited sequence, and are present in partially edited mRNAs between the 3 ′ fully edited and 5 ′ pre-edited regions. Junctions are present in >95% of RPS12 mRNAs and are hypothesized to be regions of active editing that undergo repeated remodeling (Koslowsky et al 1991;Sturm et al 1992;Ammerman et al 2010;Simpson et al 2016). TREAT designates junctions as extending from the 3 ′ most ES that does not match the fully edited sequence to the 5 ′ most editing site beyond the editing stop site that shows any editing modification.…”

Section: Effects Of Mrb7260 On Rna Editing At the Sequence Levelmentioning

confidence: 99%

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MRB7260 is essential for productive protein–RNA interactions within the RNA editing substrate binding complex during trypanosome RNA editing

McAdams

Simpson

Chen

et al. 2018

RNA

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115

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The trypanosome NAditing ubstrate bindingomplex (RESC) acts as the platform for mitochondrial uridine insertion/deletion RNA editing and facilitates the protein-protein and protein-RNA interactions required for the editing process RESC is broadly comprised of two subcomplexes: GRBC (uide NAinding omplex) and REMC (NA ditingediator omplex). Here, we characterize the function and position in RESC organization of a previously unstudied RESC protein, MRB7260. We show that MRB7260 forms numerous RESC-related complexes, including a novel, small complex with the guide RNA binding protein, GAP1, which is a canonical GRBC component, and REMC components MRB8170 and TbRGG2. RNA immunoprecipitations in MRB7260-depleted cells show that MRB7260 is critical for normal RNA trafficking between REMC and GRBC. Analysis of protein-protein interactions also reveals an important role for MRB7260 in promoting stable association of the two subcomplexes. High-throughput sequencing analysis of RPS12 mRNAs from MRB7260 replete and depleted cells demonstrates that MRB7260 is critical for gRNA exchange and early gRNA utilization, with the exception of the initiating gRNA. Together, these data demonstrate that MRB7260 is essential for productive protein-RNA interactions with RESC during RNA editing.

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Section: Effects Of Mrb7260 On Rna Editing At the Sequence Levelmentioning

confidence: 99%

Section: Effects Of Mrb7260 On Rna Editing At the Sequence Levelmentioning

confidence: 99%

Section: Effects Of Mrb7260 On Rna Editing At the Sequence Levelmentioning

confidence: 99%

Section: Effects Of Mrb7260 On Rna Editing At the Sequence Levelmentioning

confidence: 99%

See 2 more Smart Citations

MRB7260 is essential for productive protein–RNA interactions within the RNA editing substrate binding complex during trypanosome RNA editing

McAdams

Simpson

Chen

et al. 2018

RNA

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115

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“…First, many reads do not map exactly to the genomic sequence because of either somatic mutations or sequencing errors, so representing a read by the starting and ending numbers leads to loss of information. Second, RNAediting and processing can be so extensive that it becomes impossible to map a transcriptomic read to the genome (ABRAHAM et al 1988;LAMOND 1988;ALATORTSEV et al 2008;LI et al 2009;SIMPSON et al 2016). Furthermore, there are still many scientifically interesting species that do not have a good genomic sequence available.…”

Section: Converting Hts Data To Fasta+/fastq+mentioning

confidence: 99%

ARSDA: A new approach for storing, transmitting and analyzing high-throughput sequencing data

Xia

2017

Preprint

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High throughput sequencing revolution reveals conserved fundamentals of U‐indel editing

2018

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Among Euglenozoans, mitochondrial RNA editing occurs in the diplonemids and in the kinetoplastids that include parasitic trypanosomes. Yet U-indel editing, in which open reading frames (ORFs) on mRNAs are generated by insertion and deletion of uridylates in locations dictated by guide RNAs, appears confined to kinetoplastids. The nature of guide RNA and edited mRNA populations has been cursorily explored in a surprisingly extensive number of species over the years, although complete sets of fully edited mRNAs for most kinetoplast genomes are largely missing. Now, however, high throughput sequencing technologies have had an enormous impact on what we know and will learn about the mechanisms, benefits, and final edited products of U-indel editing. Tools including PARERS, TREAT, and T-Aligner function to organize and make sense of U-indel mRNA transcriptomes, which are comprised of mRNAs harboring uridylate indels both consistent and inconsistent with translatable products. From high throughput sequencing data come arguments that partially edited mRNAs containing "junction regions" of noncanonical editing are editing intermediates, and conversely, arguments that they are dead-end products. These data have also revealed that the percent of a given transcript population that is fully or partially edited varies dramatically between transcripts and organisms. Outstanding questions that are being addressed include the prevalence of sequences that apparently encode alternative ORFs, diversity of editing events in ORF termini and 5' and 3' untranslated regions, and the differences that exist in this byzantine process between species. High throughput sequencing technologies will also undoubtedly be harnessed to probe U-indel editing's evolutionary origins. This article is categorized under: RNA Processing > RNA Editing and Modification RNA Evolution and Genomics > Computational Analyses of RNA.

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High-throughput sequencing of partially edited trypanosome mRNAs reveals barriers to editing progression and evidence for alternative editing

Cited by 42 publications

References 77 publications

MRB7260 is essential for productive protein–RNA interactions within the RNA editing substrate binding complex during trypanosome RNA editing

MRB7260 is essential for productive protein–RNA interactions within the RNA editing substrate binding complex during trypanosome RNA editing

ARSDA: A new approach for storing, transmitting and analyzing high-throughput sequencing data

High throughput sequencing revolution reveals conserved fundamentals of U‐indel editing

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