Reconstitution of full-round uridine-deletion RNA editing with three recombinant proteins

Kang, Xuedong; Gao, Ge; Rogers, Kestrel; Falick, Arnold M.; Zhou, Shi-Sheng; Simpson, Larry

doi:10.1073/pnas.0604476103

Cited by 32 publications

(43 citation statements)

References 43 publications

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“…4A), indicating that TbMP42 is needed for any cleavage by the TbMP90 endonuclease in trypanosome extracts. (However, studies using recombinant proteins have shown that rTbMP90 cleaves an editing site in the presence of rTbMP63, without rTbMP42 [Kang et al 2006], suggesting that in vivo TbMP42 likely serves to retain the presence of the active TbMP90.) In contrast to its effects on the U-deletional endonuclease, depletion of TbMP42 (at 3 d of RNAi induction) does not affect the basic cleavage activity of the U-insertional endonuclease (Fig.…”

Section: Tbmp42 Is Needed Formentioning

confidence: 99%

“…In some references, the initial ''K'' is omitted, and, additionally, TbMP52 has also been referred to as DREL (Cruz-Reyes et al 2002) and TbMP48 as IREL (Cruz-Reyes et al 2002). Purification of editing complexes from L. tarentolae yields many homologous proteins, initially named LmLC# ) then shortened to LC# (Kang et al 2006). For uniformity with the bulk of the editing literature, after their initial mention, we use the TbMP# designation.…”

Section: Introductionmentioning

confidence: 99%

“…We also provide potential explanations for the previous, differing conclusions. Rusche et al (1997) (see Law et al 2007 for additional verification of the reproducibility of this purification), the ''TbMP'' designation (representing T. brucei mitochondrial protein followed by the molecular weight of its cytoplasmic precursor) from Panigrahi et al (2001a), and a more recent kinetoplastid RNA editing protein nomenclature (''KREPX#,'' representing kinetoplastid RNA editing protein followed by a letter for the class of protein and a number indicating approximate ascending size within the group), that is being replaced with a KREØ# functional nomenclature (KRE as above, followed by a letter for the biological role of protein and a number indicating approximate ascending size within the group) from the Stuart laboratory (see references in the text; for reviews, see Worthey et al 2003;Simpson et al 2004;Stuart et al 2005;Kang et al 2006;Panigrahi et al 2006). The proteins shown in brackets appear quite unabundant and/or are only obtained from some purification procedures (e.g., Panigrahi et al 2006).…”

Section: Introductionmentioning

confidence: 99%

“…1B). The U-deletional and U-insertional cleavage steps are catalyzed by TbMP90/KREN1 and TbMP61/ KREN2, respectively Trotter et al 2005;Kang et al 2006) (or by TbMP67/KREPB2/KREN3 for the U-insertion that uses a cis-located gRNA; Carnes et al 2008), although it has additionally been inferred that TbMP42/KREPA3/band VI may catalyze editing endonucleolytic cleavage (Brecht et al 2005). The U-removal step is catalyzed by TbMP100/KREX1 (Worthey et al 2003;Kang et al 2005) and TbMP99/KREPC2/KREX2/band I Worthey et al 2003;Rogers et al 2007) and/or possibly TbMP42/KREPA3/band VI (Brecht et al 2005); the U-addition step is catalyzed by the TbMP57/KRET2 TUTase (Aphasizhev et al 2003c;Ernst et al 2003).…”

Section: Introductionmentioning

confidence: 99%

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Trypanosoma brucei RNA editing protein TbMP42 (band VI) is crucial for the endonucleolytic cleavages but not the subsequent steps of U-deletion and U-insertion

Law

O’Hearn

Sollner‐Webb³

2008

RNA

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Trypanosome mitochondrial mRNAs achieve their coding sequences through RNA editing. This process, catalyzed by ;20S protein complexes, involves large numbers of uridylate (U) insertions and deletions within mRNA precursors. Here we analyze the role of the essential TbMP42 protein (band VI/KREPA2) by individually examining each step of the U-deletional and U-insertional editing cycles, using reactions in the approximately linear range. We examined control extracts and RNA interference (RNAi) extracts prepared soon after TbMP42 was depleted (when primary effects should be most evident) and three days later (when precedent shows secondary effects can become prominent). This analysis shows TbMP42 is critical for cleavage of editing substrates by both the U-deletional and U-insertional endonucleases. However, on simple substrates that assess cleavage independent of editing features, TbMP42 is similarly required only for the U-deletional endonuclease, indicating TbMP42 affects the two editing endonucleases differently. Supplementing RNAi extract with recombinant TbMP42 partly restores these cleavage activities. Notably, we find that all the other editing steps (the 39-U-exonuclease [39-U-exo] and ligation steps of U-deletion and the terminal-U-transferase [TUTase] and ligation steps of U-insertion) remain at control levels upon RNAi induction, and hence are not dependent on TbMP42. This contrasts with an earlier report that TbMP42 is a 39-U-exo that may act in U-deletion and additionally is critical for the TUTase and/or ligation steps of U-insertion, observations our data suggest reflect indirect effects of TbMP42 depletion. Thus, trypanosomes require TbMP42 for both endonucleolytic cleavage steps of RNA editing, but not for any of the subsequent steps of the editing cycles.

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Section: Tbmp42 Is Needed Formentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Trypanosoma brucei RNA editing protein TbMP42 (band VI) is crucial for the endonucleolytic cleavages but not the subsequent steps of U-deletion and U-insertion

Law

O’Hearn

Sollner‐Webb³

2008

RNA

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“…Several mRNAs are edited at over a hundred sites, and at each site, editing starts by a nuclease cleavage directed by a complementary gRNA (Rusche et al 1997;Stuart et al 2005;Li et al 2009;Simpson et al 2010). There are three accepted specialized editing endonucleases, REN1, REN2, and REN3 Trotter et al 2005;Kang et al 2006;Simpson et al 2010), although only REN1 has been produced in an active recombinant form (Kang et al 2006). RENs have a conserved RNase III domain and two domains of unknown function (Worthey et al 2003).…”

Section: Introductionmentioning

confidence: 99%

Guide RNA biogenesis involves a novel RNase III family endoribonuclease inTrypanosoma brucei

Madina¹,

Gokulan²,

Vashisht³

et al. 2011

RNA

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The mitochondrial genome of kinetoplastids, including species of Trypanosoma and Leishmania, is an unprecedented DNA structure of catenated maxicircles and minicircles. Maxicircles represent the typical mitochondrial genome encoding components of the respiratory complexes and ribosomes. However, most mRNA sequences are cryptic, and their maturation requires a unique U insertion/deletion RNA editing. Minicircles encode hundreds of small guide RNAs (gRNAs) that partially anneal with unedited mRNAs and direct the extensive editing. Trypanosoma brucei gRNAs and mRNAs are transcribed as polycistronic precursors, which undergo processing preceding editing; however, the relevant nucleases are unknown. We report the identification and functional characterization of a close homolog of editing endonucleases, mRPN1 (mitochondrial RNA precursor-processing endonuclease 1), which is involved in gRNA biogenesis. Recombinant mRPN1 is a dimeric dsRNAdependent endonuclease that requires Mg 2+ , a critical catalytic carboxylate, and generates 2-nucleotide 39 overhangs. The cleavage specificity of mRPN1 is reminiscent of bacterial RNase III and thus is fundamentally distinct from editing endonucleases, which target a single scissile bond just 59 of short duplexes. An inducible knockdown of mRPN1 in T. brucei results in loss of gRNA and accumulation of precursor transcripts (pre-gRNAs), consistent with a role of mRPN1 in processing. mRPN1 stably associates with three proteins previously identified in relatively large complexes that do not contain mRPN1, and have been linked with multiple aspects of mitochondrial RNA metabolism. One protein, TbRGG2, directly binds mRPN1 and is thought to modulate gRNA utilization by editing complexes. The proposed participation of mRPN1 in processing of polycistronic RNA and its specific protein interactions in gRNA expression are discussed.

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

et al. 2018

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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

Reconstitution of full-round uridine-deletion RNA editing with three recombinant proteins

Cited by 32 publications

References 43 publications

Trypanosoma brucei RNA editing protein TbMP42 (band VI) is crucial for the endonucleolytic cleavages but not the subsequent steps of U-deletion and U-insertion

Trypanosoma brucei RNA editing protein TbMP42 (band VI) is crucial for the endonucleolytic cleavages but not the subsequent steps of U-deletion and U-insertion

Guide RNA biogenesis involves a novel RNase III family endoribonuclease inTrypanosoma brucei

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

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