Fate of a Larch Unedited tRNA Precursor Expressed in Potato Mitochondria

Placido, Antonio; Gagliardi, Dominique; Gallerani, Raffaele; Grienenberger, Jean‐Michel; Maréchal-Drouard, Laurence

doi:10.1074/jbc.m505269200

Cited by 24 publications

(20 citation statements)

References 36 publications

(39 reference statements)

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“…These observations indicate a division of labor in A. castellanii, wherein two independent and coexisting mechanisms for tRNA His identity have evolved that are strictly compartmentalized. Inconsistencies in the occurrence of even the encoded G −1 on tRNA His have been previously reported in plant mitochondria and chloroplast (Marechal-Drouard et al 1996a,b;Placido et al 2005Placido et al , 2010.…”

Section: Discussionmentioning

confidence: 83%

Life without post-transcriptional addition of G₋₁: two alternatives for tRNA^His identity in Eukarya

Rao

Jackman

2014

RNA

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The identity of tRNAHis is strongly associated with the presence of an additional 5′-guanosine residue (G−1) in all three domains of life. The critical nature of the G−1 residue is underscored by the fact that two entirely distinct mechanisms for its acquisition are observed, with cotranscriptional incorporation observed in Bacteria, while post-transcriptional addition of G−1 occurs in Eukarya. Here, through our investigation of eukaryotes that lack obvious homologs of the post-transcriptional G−1-addition enzyme Thg1, we identify alternative pathways to tRNAHis identity that controvert these well-established rules. We demonstrate that Trypanosoma brucei, like Acanthamoeba castellanii, lacks the G−1 identity element on tRNAHis and utilizes a noncanonical G−1-independent histidyl-tRNA synthetase (HisRS). Purified HisRS enzymes from A. castellanii and T. brucei exhibit a mechanism of tRNAHis recognition that is distinct from canonical G−1-dependent synthetases. Moreover, noncanonical HisRS enzymes genetically complement the loss of THG1 in Saccharomyces cerevisiae, demonstrating the biological relevance of the G−1-independent aminoacylation activity. In contrast, in Caenorhabditis elegans, which is another Thg1-independent eukaryote, the G−1 residue is maintained, but here its acquisition is noncanonical. In this case, the G−1 is encoded and apparently retained after 5′ end processing, which has so far only been observed in Bacteria and organelles. Collectively, these observations unearth a widespread and previously unappreciated diversity in eukaryotic tRNAHis identity mechanisms.

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Section: Discussionmentioning

confidence: 83%

Life without post-transcriptional addition of G₋₁: two alternatives for tRNA^His identity in Eukarya

Rao

Jackman

2014

RNA

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“…An alternative explanation is these transcripts are recognized as mis-processed RNAs and therefore targeted to rapid degradation. Similarly, PNPase probably degrades other type of misprocessed RNAs such as misfolded tRNA precursors (Placido et al 2005). However, specific quality-control mechanism that monitors for example mRNA editing appear to be absent in plant mitochondria (Holec et al 2008a) Another role of PNPase is the elimination of tRNA and rRNA maturation by-products (Holec et al 2006).…”

Section: Rna Degradation Shapes the Transcriptome Of Plant Mitochondriamentioning

confidence: 99%

Polyadenylation in RNA Degradation Processes in Plants

Lange

Gagliardi

2011

RNA Technologies

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Although polyadenylation is best known for stabilizing eukaryotic mRNAs and promoting their translation, the primordial role of polyadenylation is to target RNAs for degradation by 3¢→5¢ exoribonucleases. This ancient mechanism is conserved among bacteria and eukaryotes, and in plants, polyadenylation-assisted RNA degradation operates in the nucleus, the chloroplast, and the mitochondrion. Polyadenylation-assisted RNA degradation contributes to maturation, turnover, and quality control of a variety of transcripts, the nature of which varies in the different genetic compartments of the plant cell. Moreover, polyadenylation-assisted RNA degradation rapidly removes a large variety of novel transcripts of unknown function that are produced by extensive transcription of extragenic regions, in particular from nuclear and mitochondrial genomes. In this chapter, we review the current knowledge of polyadenylation-assisted RNA degradation in plants, highlighting the different impact of this RNA degradation pathway on the expression of nuclear, plastidial, or mitochondrial genomes.

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“…vulgare total nucleic acid was first treated with DNASE RQ1 according to manufacturer's intructions (Promega). The DNase-treated RNA sample was then used as substrate for RT-PCR amplification using relevant pairs of primers, cloned into pGEM-T Easy (Promega), as described in 51 and sequenced.…”

Section: Cloning Of Reverse Transcription (Rt)-pcr Productsmentioning

confidence: 99%

“…51 Briefly, total RNA extracted from A. vulgare was incubated with 40U of T4 RNA ligase (New England Biolabs) in the supplied buffer supplemented with 2U of RNase inhibitor and in a total volume of 25 ml. Following circularization, all steps of RT-PCR were classically carried out using a relevant pair of primers.…”

Section: Cloning Of Reverse Transcription (Rt)-pcr Productsmentioning

confidence: 99%

Large gene overlaps and tRNA processing in the compact mitochondrial genome of the crustaceanArmadillidium vulgare

et al. 2015

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Fate of a Larch Unedited tRNA Precursor Expressed in Potato Mitochondria

Cited by 24 publications

References 36 publications

Life without post-transcriptional addition of G₋₁: two alternatives for tRNA^His identity in Eukarya

Life without post-transcriptional addition of G₋₁: two alternatives for tRNA^His identity in Eukarya

Polyadenylation in RNA Degradation Processes in Plants

Large gene overlaps and tRNA processing in the compact mitochondrial genome of the crustaceanArmadillidium vulgare

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Fate of a Larch Unedited tRNA Precursor Expressed in Potato Mitochondria

Cited by 24 publications

References 36 publications

Life without post-transcriptional addition of G−1: two alternatives for tRNAHis identity in Eukarya

Life without post-transcriptional addition of G−1: two alternatives for tRNAHis identity in Eukarya

Polyadenylation in RNA Degradation Processes in Plants

Large gene overlaps and tRNA processing in the compact mitochondrial genome of the crustaceanArmadillidium vulgare

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Product

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Life without post-transcriptional addition of G₋₁: two alternatives for tRNA^His identity in Eukarya

Life without post-transcriptional addition of G₋₁: two alternatives for tRNA^His identity in Eukarya