2011
DOI: 10.1073/pnas.1014152108
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Trypanosome REH1 is an RNA helicase involved with the 3′–5′ polarity of multiple gRNA-guided uridine insertion/deletion RNA editing

Abstract: Uridine insertion/deletion RNA editing in kinetoplastid mitochondria corrects encoded frameshifts in mRNAs. The genetic information for editing resides in small guide RNAs (gRNAs), which form anchor duplexes just downstream of an editing site and mediate editing within a single editing "block." Many mRNAs require multiple gRNAs; the observed overall 3′ to 5′ polarity of editing is determined by the formation of upstream mRNA anchors by downstream editing. Hel61, a mitochondrial DEAD-box protein, was previously… Show more

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Cited by 52 publications
(57 citation statements)
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“…Whether or not this activity affects editing substrate binding to other MRBs needs to be examined. REH2-dependent unwinding could also control global intra-strand mRNA structure or gRNA exchange during editing progression, as it was proposed for TbRGG2 and REH1, respectively (Ammerman et al 2010;Li et al 2011). It was proposed that RNAi-repression of REH2 reduces gRNA stability (Hashimi et al 2009).…”
Section: Discussionmentioning
confidence: 99%
“…Whether or not this activity affects editing substrate binding to other MRBs needs to be examined. REH2-dependent unwinding could also control global intra-strand mRNA structure or gRNA exchange during editing progression, as it was proposed for TbRGG2 and REH1, respectively (Ammerman et al 2010;Li et al 2011). It was proposed that RNAi-repression of REH2 reduces gRNA stability (Hashimi et al 2009).…”
Section: Discussionmentioning
confidence: 99%
“…Resolution of both inter-and intramolecular RNA structure has long been recognized as essential for proper 3 ′ to 5 ′ progression of editing, and several protein factors that may contribute to this process have been described. These include the helicases REH1 (Li et al 2011) and REH2 (Hernandez et al 2010;Madina et al 2014Madina et al , 2015, the 6A). The bottom panel shows the abundance of pausing at each editing site in RPS12 (replicate 1), and intrinsic pause sites are denoted by an asterisk (from Fig.…”
Section: Discussionmentioning
confidence: 99%
“…That gRNA then needs to be at least partially removed because the subsequent gRNA forms an anchor duplex with a portion of the edited region guided by the first gRNA (Maslov and Simpson 1992). The mechanism of gRNA exchange is poorly understood, but may involve mitochondrial helicases (Hernandez et al 2010;Li et al 2011;Madina et al 2014Madina et al , 2015. This gRNA utilization process proceeds throughout the length of a given mRNA, resulting in the general, although not precise, progression of editing from the 3 ′ to the 5 ′ end of the transcript (Sturm and Simpson 1990;Koslowsky et al 1991;Souza et al 1992).…”
Section: Introductionmentioning
confidence: 99%
“…The anchor helix and U-helix may keep the gRNA's template sequence bound to the premRNA after cleavage of the pre-mRNA during editing, and thereby keep the two internal ends of the cleaved mRNA in close proximity for religation (Koslowsky et al 2004). After the editosome has finished using the template domain of a particular gRNA, a RNA editing-specific helicase (Li et al 2011) displaces the gRNA strand from the mRNA, a different gRNA binds to the next ABS 59 to the last editing site on the mRNA, and the editing reaction cycles continue.…”
Section: Introductionmentioning
confidence: 99%