<i>Arabidopsis</i> tRNA Adenosine Deaminase Arginine Edits the Wobble Nucleotide of Chloroplast tRNAArg(ACG) and Is Essential for Efficient Chloroplast Translation

Delannoy, Étienne; Ret, Monique Le; Faivre-Nitschke, Emmanuelle; Estavillo, Gonzalo M.; Bergdoll, Marc; Taylor, Nicolas L.; Pogson, Barry J.; Small, Ian; Imbault, P.; Gualberto, José M.

doi:10.1105/tpc.109.066654

Cited by 66 publications

(80 citation statements)

References 53 publications

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“…1). Construction of an evolutionary tree from all putative nucleoside deaminases encoded in the Arabidopsis nuclear genome (Arabidopsis Genome Initiative, 2000) revealed several additional proteins with similarity to the two functionally characterized A-to-I deaminases, TADA and TAD1 (Delannoy et al, 2009;Karcher and Bock, 2009;Zhou et al, 2013). We preliminarily designated these proteins AtTAD2, AtTAD3, AtTAD4, and AtTAD5 (for simplicity, subsequently referred to as TAD2, TAD3, TAD4, and TAD5; Fig.…”

Section: Identification Of Putative Adenosine Deaminases In the Arabimentioning

confidence: 99%

“…The specific adenosine deaminase conducting this conversion (termed tadA, for tRNAspecific adenosine deaminase) is an essential enzyme, and inactivation of the tadA gene is lethal, presumably because of the requirement for inosine in the wobble position to read the three Arg codons CGU, CGC, and CGA. A tadA homolog exists in chloroplasts (plastids) of plants and generates inosine-34 in the same tRNA species, tRNA-Arg(ACG) (Delannoy et al, 2009;Karcher and Bock, 2009). Interestingly, the gene encoding the plant tadA homolog (TADA) is not essential, even though plastid protein biosynthesis (Ahlert et al, 2003;Rogalski et al, 2006Rogalski et al, , 2008bFleischmann et al, 2011) and most plastid tRNA species (Rogalski et al, 2008a;Alkatib et al, 2012aAlkatib et al, , 2012b) are known to be essential for cell survival.…”

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Identification of Enzymes for Adenosine-to-Inosine Editing and Discovery of Cytidine-to-Uridine Editing in Nucleus-Encoded Transfer RNAs of Arabidopsis

2014

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In all organisms, transfer RNAs (tRNAs) contain numerous modified nucleotides. For many base modifications in tRNAs, the functional significance is not well understood, and the enzymes performing the modification reactions are unknown. Here, we have studied members of a family of putative nucleotide deaminases in the model plant Arabidopsis (Arabidopsis thaliana). We show that two Arabidopsis genes encoding homologs of yeast (Saccharomyces cerevisiae) tRNA adenosine deaminases catalyze adenosine-to-inosine editing in position 34 of several cytosolic tRNA species. The encoded proteins (AtTAD2 and AtTAD3, for tRNA-specific adenosine deaminase) localize to the nucleus and interact with each other in planta in bimolecular fluorescence complementation and coimmunoprecipitation assays. Both AtTAD2 and AtTAD3 are encoded by essential genes whose knockout is lethal and leads to arrested embryo development at the globular stage. Knockdown mutants for AtTAD2 and AtTAD3 display reduced growth and inefficient editing from adenosine to inosine in six nucleus-encoded tRNA species. Moreover, upon comparison of DNA and complementary DNA sequences, we discovered cytidine-to-uridine RNA editing in position 32 of two nucleus-encoded serine tRNAs, tRNA-serine(AGA) and tRNA-serine(GCT). This adds a unique type of RNA editing to the modifications occurring in nuclear genome-encoded RNAs in plants.

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Section: Identification Of Putative Adenosine Deaminases In the Arabimentioning

confidence: 99%

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confidence: 99%

Identification of Enzymes for Adenosine-to-Inosine Editing and Discovery of Cytidine-to-Uridine Editing in Nucleus-Encoded Transfer RNAs of Arabidopsis

2014

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“…These are encoded by the loci At5g28050, At1g68720, At3g05300, At1g48175, and At4g20960 (in order of decreasing similarity). Some of these could be excluded as GDA candidate loci because they were already functionally characterized: The locus At4g20960 was previously shown to code for a deaminase involved in riboflavin biosynthesis (Fischer et al, 2004), and At1g68720 codes for the chloroplastic tRNA adenosine deaminase Arg (Delannoy et al, 2009;Karcher and Bock, 2009). The locus At1g48175 encodes an uncharacterized protein that is highly conserved in plants.…”

Section: Identification Of Gsda From a Thalianamentioning

confidence: 99%

Plant Purine Nucleoside Catabolism Employs a Guanosine Deaminase Required for the Generation of Xanthosine in Arabidopsis

Dahncke

Witte

2013

Plant Cell

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“…Inosine has not been described in mitochondria, but a recent report showed that a bacteria-type ADATa enzyme plays key functions in inosine formation and thus translation in chloroplasts (16,17). ADATa only targets a single tRNA (tRNA ACG Arg ) and can efficiently catalyze deamination of an anticodon stem loop corresponding to a minimal version of tRNA ACG Arg (4).…”

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A Single Zinc Ion Is Sufficient for an Active Trypanosoma brucei tRNA Editing Deaminase

Spears

Rubio

Gaston

et al. 2011

Journal of Biological Chemistry

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Editing of adenosine (A) to inosine (I) at the first anticodon position in tRNA is catalyzed by adenosine deaminases acting on tRNA (ADATs). This essential reaction in bacteria and eukarya permits a single tRNA to decode multiple codons. Bacterial ADATa is a homodimer with two bound essential Zn 2؉ . The ADATa crystal structure revealed residues important for substrate binding and catalysis; however, such high resolution structural information is not available for eukaryotic tRNA deaminases. Despite significant sequence similarity among deaminases, we continue to uncover unexpected functional differences between Trypanosoma brucei ADAT2/3 (TbADAT2/3) and its bacterial counterpart. Previously, we demonstrated that TbADAT2/3 is unique in catalyzing two different deamination reactions. Here we show by kinetic analyses and inductively coupled plasma emission spectrometry that wild type TbADAT2/3 coordinates two Zn 2؉ per heterodimer, but unlike any other tRNA deaminase, mutation of one of the key Zn 2؉ -coordinating cysteines in TbADAT2 yields a functional enzyme with a singlebound zinc. These data suggest that, at least, TbADAT3 may play a role in catalysis via direct coordination of the catalytic Zn 2؉ . These observations raise the possibility of an unusual Zn 2؉ coordination interface with important implications for the function and evolution of editing deaminases.

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Arabidopsis tRNA Adenosine Deaminase Arginine Edits the Wobble Nucleotide of Chloroplast tRNAArg(ACG) and Is Essential for Efficient Chloroplast Translation

Cited by 66 publications

References 53 publications

Identification of Enzymes for Adenosine-to-Inosine Editing and Discovery of Cytidine-to-Uridine Editing in Nucleus-Encoded Transfer RNAs of Arabidopsis

Identification of Enzymes for Adenosine-to-Inosine Editing and Discovery of Cytidine-to-Uridine Editing in Nucleus-Encoded Transfer RNAs of Arabidopsis

Plant Purine Nucleoside Catabolism Employs a Guanosine Deaminase Required for the Generation of Xanthosine in Arabidopsis

A Single Zinc Ion Is Sufficient for an Active Trypanosoma brucei tRNA Editing Deaminase

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