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

McAdams, Natalie M.; Simpson, Rachel M.; Chen, Runpu; Sun, Yijun; Read, Laurie K.

doi:10.1261/rna.065169.117

Cited by 23 publications

(122 citation statements)

References 54 publications

Supporting

Mentioning

115

Contrasting

Order By: Relevance

“…This includes COII mRNA, whose editing does not depend on trans-acting gRNAs or GAP1/ 2. Because the effects of editing factor depletion are typically more dramatic on pan-edited than on minimally edited mRNAs (Fisk et al 2008;Acestor et al 2009;Ammerman et al 2011Ammerman et al , 2013Huang et al 2015;Simpson et al 2017;McAdams et al 2018), these data suggest a distinct and fundamental function for MRB10130. To determine whether the MRB10130 impact on editing could involve direct RNA binding, we performed UV cross-linking assays with recombinant MRB10130 and body-labeled gRNA or mRNA.…”

Section: Resultsmentioning

confidence: 92%

“…We can then further analyze editing progression by determining the editing stop site in each mRNA, which is defined as the final (5 ′ most) ES that matches the canonical fully edited sequence correctly (Table 1; Simpson et al 2016). At a population level, TREAT allows us to define exacerbated pause sites (EPSs; Table 1); EPSs are editing stop sites at which canonical editing pauses to a significant extent in a given knockdown cell line compared to uninduced controls (P < 0.05, q < 0.05) (Simpson et al 2017;McAdams et al 2018;Tylec et al 2019). Additionally, we can analyze the lengths and sequences of misedited junctions 5 ′ of EPSs to provide insights into specific editing defects that arise when distinct editing factors are depleted (Table 1; Simpson et al 2017;McAdams et al 2018;Tylec et al 2019).…”

Section: Sequence Level Analysis Of Rna Editing Defects In Mrb10130 Kmentioning

confidence: 99%

“…Early proteomic and yeast two-hybrid studies identified two modules comprising RESC, the guide RNA binding complex (GRBC) and the RNA editing mediator complex (REMC), that appear to associate in a dynamic fashion mediated in part by protein-RNA interactions (Ammerman et al 2012;Aphasizheva et al 2014). More recent studies point to the existence of numerous variants of RESC (Kafkova et al 2012;Madina et al 2015;Simpson et al 2017;McAdams et al 2018), and the organization and functions of RESC are a subject of ongoing research.…”

Section: Introductionmentioning

confidence: 99%

“…For example, the founding and defining component of this complex is the GAP1/2 heterotetramer, which is essential for stability of the entire gRNA population (Weng et al 2008;Hashimi et al 2009;Kumar et al 2016). GAP1/2 is canonically referred to as a component of the GRBC module; however, it has now been identified in small complexes apart from fully assembled RESC that contain either REH2, TbRGG3, or MRB7260, indicating a broader function for this protein than first appreciated (Madina et al 2014;McAdams et al 2015McAdams et al , 2018. Several components of the REMC module have been studied using biochemical assays, domain interaction and protein-RNA interaction studies, and high-throughput sequencing (HTS), in one case combined with in vivo protein-RNA crosslinking.…”

Section: Introductionmentioning

confidence: 99%

“…We recently showed that the RESC component, MRB7260, plays a role in modulating GRBC-REMC interactions within the RESC complex during editing (McAdams et al 2018). Depletion of MRB7260 caused dissociation of GRBC and REMC, with concomitant disruption of normal mRNA and gRNA trafficking within RESC.…”

Section: Introductionmentioning

confidence: 99%

See 4 more Smart Citations

MRB10130 is a RESC assembly factor that promotes kinetoplastid RNA editing initiation and progression

McAdams

Harrison

Tylec

et al. 2019

RNA

Self Cite

View full text Add to dashboard Cite

Uridine insertion deletion editing in kinetoplastid protozoa requires a complex machinery, a primary component of which is the RNA editing substrate binding complex (RESC). RESC contains two modules termed GRBC (guide RNA binding complex) and REMC (RNA editing mediator complex), although how interactions between these modules and their mRNA and gRNA binding partners are controlled is not well understood. Here, we demonstrate that the ARM/HEAT repeat containing RESC protein, MRB10130, controls REMC association with mRNA-and gRNA-loaded GRBC. High-throughput sequencing analyses show that MRB10130 functions in both initiation and 3 ′ ′ ′ ′ ′ to 5 ′ ′ ′ ′ ′ progression of editing through gRNA-defined domains. Editing intermediates that accumulate upon MRB10130 depletion significantly intersect those in cells depleted of another RESC organizer, MRB7260, but are distinct from those in cells depleted of specific REMC proteins. We present a model in which MRB10130 coordinates numerous protein-protein and protein-RNA interactions during editing progression.

show abstract

Section: Resultsmentioning

confidence: 92%

Section: Sequence Level Analysis Of Rna Editing Defects In Mrb10130 Kmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 3 more Smart Citations

MRB10130 is a RESC assembly factor that promotes kinetoplastid RNA editing initiation and progression

McAdams

Harrison

Tylec

et al. 2019

RNA

Self Cite

View full text Add to dashboard Cite

show abstract

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

2018

Self Cite

View full text Add to dashboard Cite

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.

show abstract

Dynamic RNA holo‐editosomes with subcomplex variants: Insights into the control of trypanosome editing

et al. 2018

View full text Add to dashboard Cite

RNA editing causes massive remodeling of the mitochondrial mRNA transcriptome in trypanosomes and related kinetoplastid protozoa. This type of editing involves the specific insertion or deletion of uridylates (U) directed by small noncoding guide RNAs (gRNAs). Because U-insertion exceeds U-deletion by a factor of 10, editing increases the nascent mRNA size by up to 55%. In Trypanosoma brucei, the editing apparatus uses ~40 proteins and >1,200 gRNAs to create the functional open reading frame in 12 mRNAs. Thousands of sites are specifically recognized in the pre-edited mRNAs and a myriad of partially edited transcript intermediates accumulates in mitochondria. The control of editing is poorly understood, but past work suggests that it occurs during substrate recognition, the initiation and progression of editing, and during the life-cycle in different hosts. The growing understanding of the editing proteins offers clues about editing control. Most editing proteins reside in the "RNA-free" RNA editing core complex (RECC) and in the accessory RNA editing substrate complex (RESC) that contains gRNA. Two accessory RNA helicases are known, including one in the RNA editing helicase 2 complex (REH2C). Both the RESC and the REH2C associate with mRNA, providing a rationale for the assembly of mRNA or its mRNPs, RESC, and the RECC enzyme. Identified variants of the canonical editing complexes further complicate the model of RNA editing. We examine specific examples of complex variants, differential effects of editing proteins on the mRNAs within and between T. brucei life stages, and possible control points in RNA holo-editosomes. This article is categorized under: RNA Processing > RNA Editing and Modification RNA Interactions with Proteins and Other Molecules > RNA-Protein Complexes RNA Interactions with Proteins and Other Molecules > Protein-RNA Interactions: Functional Implications.

show abstract

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

Cited by 23 publications

References 54 publications

MRB10130 is a RESC assembly factor that promotes kinetoplastid RNA editing initiation and progression

MRB10130 is a RESC assembly factor that promotes kinetoplastid RNA editing initiation and progression

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

Dynamic RNA holo‐editosomes with subcomplex variants: Insights into the control of trypanosome editing

Contact Info

Product

Resources

About