Detection of a Subset of Posttranscriptional Transfer RNA Modifications <i>in Vivo</i> with a Restriction Fragment Length Polymorphism-Based Method

Wulff, Thomas F.; Argüello, Rafael J.; Jordàn, Marc Molina; Frigolé, Helena Roura; Hauquier, Glenn; Filonava, Liudmila; Camacho, Noelia; Gatti, Evelina; Pierre, Philippe; Pouplana, Lluı́s Ribas de; Torres, Adrián Gabriel

doi:10.1021/acs.biochem.7b00324

Cited by 12 publications

(13 citation statements)

References 36 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…2B, Valine-AAC, children II:1 and II:2). The presence of the C peak is due to tRNA-Val-CAC, which is nearly identical to tRNA-Val-AAC and is recognized by the same oligos used for RT-PCR amplification (Wulff et al 2017). We also detected a similar decrease in inosine modification when examining the sequencing chromatograms of tRNA-Pro-AGG.…”

Section: Individuals Harboring the Compound Adat3 Variants Exhibit Decreased Wobble Inosine Modification In Trnasupporting

confidence: 52%

“…As additional verification for reduced wobble inosine modification, we monitored wobble inosine status in specific tRNAs using RT-PCR sequencing. Since inosine is a guanosine (G) analog, the presence of inosine can be detected by sequencing of cDNA products generated by RT-PCR of cellular tRNA (Motorin et al 2007;Kawahara 2012;Wulff et al 2017). Using this strategy, we measured the wobble inosine status of tRNA-Val-AAC and tRNA-Pro-AGG in the fibroblast cell lines.…”

Section: Individuals Harboring the Compound Adat3 Variants Exhibit Decreased Wobble Inosine Modification In Trnamentioning

confidence: 99%

See 1 more Smart Citation

Identification and rescue of a tRNA wobble inosine deficiency causing intellectual disability disorder

Ramos

Proven

Halvardson

et al. 2020

RNA

View full text Add to dashboard Cite

The deamination of adenosine to inosine at the wobble position of tRNA is an essential post-transcriptional RNA modification required for wobble decoding in bacteria and eukaryotes. In humans, the wobble inosine modification is catalyzed by the heterodimeric ADAT2/3 complex. Here, we describe novel pathogenic ADAT3 variants impairing adenosine deaminase activity through a distinct mechanism that can be corrected through expression of the heterodimeric ADAT2 subunit. The variants were identified in a family in which all three siblings exhibit intellectual disability linked to biallelic variants in the ADAT3 locus. The biallelic ADAT3 variants result in a missense variant converting alanine to valine at a conserved residue or the introduction of a premature stop codon in the deaminase domain. Fibroblast cells derived from two ID-affected individuals exhibit a reduction in tRNA wobble inosine levels and severely diminished adenosine tRNA deaminase activity. Notably, the ADAT3 variants exhibit impaired interaction with the ADAT2 subunit and alterations in ADAT2-dependent nuclear localization. Based upon these findings, we find that tRNA adenosine deaminase activity and wobble inosine modification can be rescued in patient cells by overexpression of the ADAT2 catalytic subunit. These results uncover a key role for the inactive ADAT3 deaminase domain in proper assembly with ADAT2 and demonstrate that ADAT2/3 nuclear import is required for maintaining proper levels of the wobble inosine modification in tRNA.

show abstract

Section: Individuals Harboring the Compound Adat3 Variants Exhibit Decreased Wobble Inosine Modification In Trnasupporting

confidence: 52%

Section: Individuals Harboring the Compound Adat3 Variants Exhibit Decreased Wobble Inosine Modification In Trnamentioning

confidence: 99%

Identification and rescue of a tRNA wobble inosine deficiency causing intellectual disability disorder

Ramos

Proven

Halvardson

et al. 2020

RNA

View full text Add to dashboard Cite

show abstract

“…This procedure, by avoiding the retrotranscription of the anticodon, limits the identification of different isodecoders. Also, by RFLP (restriction fragment length polymorphism) studies, different post-transcriptional modifications at specific sites of different tRNA types have been detected, taking advantage of the fact that base changes on reverse transcription PCR amplicons generated as a consequence of posttranscriptional modifications might create or abolish endonuclease restriction sites (Wulff et al 2017).…”

Section: The State Of the Trna Population In The Cellmentioning

confidence: 99%

Protein folding and tRNA biology

2017

View full text Add to dashboard Cite

Polypeptides can fold into tertiary structures while they are synthesized by the ribosome. In addition to the amino acid sequence, protein folding is determined by several factors within the cell. Among others, the folding pathway of a nascent polypeptide can be affected by transient interactions with other proteins, ligands, or the ribosome, as well as by the translocation through membrane pores. Particularly, the translation machinery and the population of tRNA under different physiological or adaptive responses can dramatically affect protein folding. This review summarizes the scientific evidence describing the role of translation kinetics and tRNA populations on protein folding and addresses current efforts to better understand tRNA biology. It is organized into three main parts, which are focused on: (i) protein folding in the cellular context; (ii) tRNA biology and the complexity of the tRNA population; and (iii) available methods and technical challenges in the characterization of tRNA pools. In this manner, this work illustrates the ways by which functional properties of proteins may be modulated by cellular tRNA populations.

show abstract

“…We then performed inhibition assays of ADAT-dependent deamination using tRNA fragments, to determine if the mode of tRNA recognition by ADAT is equivalent between human tRNA Arg ACG and tRNA Ala AGC . Using the RFLP method (Wulff et al 2017) we examined I34 formation in tRNA Arg ACG (3 µM) in the presence of 50 µM tRNA Ala AGC fragments, and vice versa (Fig. 4).…”

Section: The Substrate Recognition Mode Of Adat Varies Between Different Trnasmentioning

confidence: 99%

tRNA deamination by ADAT requires substrate-specific recognition mechanisms and can be inhibited by tRFs

Frigolé

Camacho

Coma

et al. 2019

RNA

Self Cite

View full text Add to dashboard Cite

Adenosine deaminase acting on transfer RNA (ADAT) is an essential eukaryotic enzyme that catalyzes the deamination of adenosine to inosine at the first position of tRNA anticodons. Mammalian ADATs modify eight different tRNAs, having increased their substrate range from a bacterial ancestor that likely deaminated exclusively tRNA Arg . Here we investigate the recognition mechanisms of tRNA Arg and tRNA Ala by human ADAT to shed light on the process of substrate expansion that took place during the evolution of the enzyme. We show that tRNA recognition by human ADAT does not depend on conserved identity elements, but on the overall structural features of tRNA. We find that ancestral-like interactions are conserved for tRNA Arg , while eukaryote-specific substrates use alternative mechanisms. These recognition studies show that human ADAT can be inhibited by tRNA fragments in vitro, including naturally occurring fragments involved in important regulatory pathways.

show abstract

Detection of a Subset of Posttranscriptional Transfer RNA Modifications in Vivo with a Restriction Fragment Length Polymorphism-Based Method

Cited by 12 publications

References 36 publications

Identification and rescue of a tRNA wobble inosine deficiency causing intellectual disability disorder

Identification and rescue of a tRNA wobble inosine deficiency causing intellectual disability disorder

Protein folding and tRNA biology

tRNA deamination by ADAT requires substrate-specific recognition mechanisms and can be inhibited by tRFs

Contact Info

Product

Resources

About