In vivo analysis of trypanosome mitochondrial RNA function by artificial site-specific RNA endonuclease-mediated knockdown

Szempruch, Anthony J.; Choudhury, Rajarshi; Wang, Zefeng; Hajduk, Stephen L.

doi:10.1261/rna.052084.115

Cited by 6 publications

(7 citation statements)

References 49 publications

(68 reference statements)

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“…If the dual-coding ARFs give BF trypanosomes a selective growth advantage similar to that observed by the COIII alternative protein AEP1, then the number of “essential” gRNA genes would increase greatly. Currently, only AEP1, A6 and RPS12 mitochondrial genes have been experimentally shown to be essential [12, 70-71]. In addition, the presence of alternative editing and dual-coding genes would complement the protection provided by gene fragmentation by also shielding the genes from deleterious point mutations within critical ETC genes.…”

Section: Discussionmentioning

confidence: 99%

Mitochondrial Dual-coding Genes inTrypanosomabrucei

Kirby

Koslowsky

2017

Preprint

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13Trypanosoma brucei is transmitted between mammalian hosts by the tsetse fly. In the mammal, they 14 genes may be dual-coding and that RNA editing allows access to both reading frames. We 27 hypothesize that dual-coding genes can protect genetic information by essentially hiding a non-28 selected gene within one that remains under selection. Thus, the complex RNA editing system 29 found in the mitochondria of trypanosomes provides a unique molecular strategy to combat genetic 30 drift in non-selective conditions.

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Section: Discussionmentioning

confidence: 99%

Mitochondrial Dual-coding Genes inTrypanosomabrucei

Kirby

Koslowsky

2017

Preprint

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“…The full coverage of COIII was also not surprising, as COIII was shown to be fully edited and equally abundant in both stages [ 17 ]. However, we expected to see complete coverage of ATPase 6 and RPS12 as both of these transcripts have been shown to be essential in both life cycle stages [ 3 , 44 , 45 , 50 ]. For ATPase 6, we did identify a total of 29 gRNA populations that do cover all of the editing sites.…”

Section: Discussionmentioning

confidence: 99%

Analysis of the Trypanosoma brucei EATRO 164 Bloodstream Guide RNA Transcriptome

et al. 2016

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The mitochondrial genome of Trypanosoma brucei contains many cryptogenes that must be extensively edited following transcription. The RNA editing process is directed by guide RNAs (gRNAs) that encode the information for the specific insertion and deletion of uridylates required to generate translatable mRNAs. We have deep sequenced the gRNA transcriptome from the bloodstream form of the EATRO 164 cell line. Using conventionally accepted fully edited mRNA sequences, ~1 million gRNAs were identified. In contrast, over 3 million reads were identified in our insect stage gRNA transcriptome. A comparison of the two life cycle transcriptomes show an overall ratio of procyclic to bloodstream gRNA reads of 3.5:1. This ratio varies significantly by gene and by gRNA populations within genes. The variation in the abundance of the initiating gRNAs for each gene, however, displays a trend that correlates with the developmental pattern of edited gene expression. A comparison of related major classes from each transcriptome revealed a median value of ten single nucleotide variations per gRNA. Nucleotide variations were much less likely to occur in the consecutive Watson-Crick anchor region, indicating a very strong bias against G:U base pairs in this region. This work indicates that gRNAs are expressed during both life cycle stages, and that differential editing patterns observed for the different mitochondrial mRNA transcripts are not due to the presence or absence of gRNAs. However, the abundance of certain gRNAs may be important in the developmental regulation of RNA editing.

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“…Furthermore, northern blot analysis of total RNA showed that cytoplasmic RNAs containing perfect or nearperfect eight-nucleotide sequences were not cleaved, which strongly suggests that A6-ASRE only cleaved mtRNA targets, and is thus highly specific. Measurements of mitochondrial membrane potential (ΔΨm) also confirmed that mitochondrial activity was reduced upon A6-ASRE induction, causing a 100fold increase in sensitivity to oligomycin, an ATP synthase inhibitor [112].…”

Section: (C) Targeted Mtrna Nucleasesmentioning

confidence: 77%

“…The authors attributed this to inadequate protein import or low transfection efficiency, while stable cell lines producing mitoASREs enabled a reduction of 70% in MT-ND5 mRNA [110]. Further work by Choudhury and co-workers expanded the PUF-PIN ASRE system to target and knock-down specific mtRNAs of Trypanosoma brucei [112]. Trypanosomes are parasitic protists with a host life cycle that rotates between insect vectors, such as the tsetse fly, and mammals, specifically cattle, where they cause African sleeping sickness [113].…”

Section: (C) Targeted Mtrna Nucleasesmentioning

confidence: 99%

“…This process involves the insertion or deletion of out-of-frame uridines to produce complete open reading frames [116,117]. To study the function of mtRNAs in kinetoplastids, synthetic PUF-PIN proteins were designed to target a specific GUUAUUGG sequence in the 3 0 -UTR of the edited transcript of the A6 subunit of the mitochondrial FoF1-ATPase [112]. These PUF-PIN proteins contained an N-terminal MTS from dihydroplipoyl dehydrogenase [118].…”

Section: (C) Targeted Mtrna Nucleasesmentioning

confidence: 99%

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Manipulating and elucidating mitochondrial gene expression with engineered proteins

Wallis

Scott

Filipovska

et al. 2019

Phil. Trans. R. Soc. B

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Many conventional, modern genome engineering tools cannot be used to study mitochondrial genetics due to the unusual structure and physiology of the mitochondrial genome. Here, we review a number of newly developed, synthetic biology-based approaches for altering levels of mutant mammalian mitochondrial DNA and mitochondrial RNAs, including transcription activator-like effector nucleases, zinc finger nucleases and engineered RNA-binding proteins. These approaches allow researchers to manipulate and visualize mitochondrial processes and may provide future therapeutics. This article is part of the theme issue ‘Linking the mitochondrial genotype to phenotype: a complex endeavour’.

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In vivo analysis of trypanosome mitochondrial RNA function by artificial site-specific RNA endonuclease-mediated knockdown

Cited by 6 publications

References 49 publications

Mitochondrial Dual-coding Genes inTrypanosomabrucei

Mitochondrial Dual-coding Genes inTrypanosomabrucei

Analysis of the Trypanosoma brucei EATRO 164 Bloodstream Guide RNA Transcriptome

Manipulating and elucidating mitochondrial gene expression with engineered proteins

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