Pseudouridine in the Anticodon of Escherichia coli tRNATyr(QΨA) Is Catalyzed by the Dual Specificity Enzyme RluF

Addepalli, Balasubrahmanyam; Limbach, Patrick A.

doi:10.1074/jbc.m116.747865

Cited by 38 publications

(39 citation statements)

References 61 publications

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“…The archaeal Pus10 protein (MJ0041) generates ⌿54 and ⌿55 in archaeal tRNAs (58), although pseudouridine at position 55 can also be generated through an H/ACA guide RNA mechanism (59-62). As no pseudouridine-specific mapping was performed (63,64), the localization of this modification to positions 54 and 55 of specific tRNAs is expected but not verified here. The DUF358 SPOUT-methyltransferase MJ1640 (renamed TrmY) acts in concert with Pus10 to catalyze the biosynthesis of m 1 ⌿ at position 54 (65)(66)(67).…”

Section: Discussionmentioning

confidence: 66%

tRNA Modification Profiles and Codon-Decoding Strategies in Methanocaldococcus jannaschii

Jora

Solivio

et al. 2019

J Bacteriol

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tRNAs play a critical role in mRNA decoding, and posttranscriptional modifications within tRNAs drive decoding efficiency and accuracy. The types and positions of tRNA modifications in model bacteria have been extensively studied, and tRNA modifications in a few eukaryotic organisms have also been characterized and localized to particular tRNA sequences. However, far less is known regarding tRNA modifications in archaea. While the identities of modifications have been determined for multiple archaeal organisms, Haloferax volcanii is the only organism for which modifications have been extensively localized to specific tRNA sequences. To improve our understanding of archaeal tRNA modification patterns and codondecoding strategies, we have used liquid chromatography and tandem mass spectrometry to characterize and then map posttranscriptional modifications on 34 of the 35 unique tRNA sequences of Methanocaldococcus jannaschii. A new posttranscriptionally modified nucleoside, 5-cyanomethyl-2-thiouridine (cnm 5 s 2 U), was discovered and localized to position 34. Moreover, data consistent with wyosine pathway modifications were obtained beyond the canonical tRNA Phe as is typical for eukaryotes. The high-quality mapping of tRNA anticodon loops enriches our understanding of archaeal tRNA modification profiles and decoding strategies. IMPORTANCE While many posttranscriptional modifications in M. jannaschii tRNAs are also found in bacteria and eukaryotes, several that are unique to archaea were identified. By RNA modification mapping, the modification profiles of M. jannaschii tRNA anticodon loops were characterized, allowing a comparative analysis with H. volcanii modification profiles as well as a general comparison with bacterial and eukaryotic decoding strategies. This general comparison reveals that M. jannaschii, like H. volcanii, follows codon-decoding strategies similar to those used by bacteria, although position 37 appears to be modified to a greater extent than seen in H. volcanii.

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Section: Discussionmentioning

confidence: 66%

tRNA Modification Profiles and Codon-Decoding Strategies in Methanocaldococcus jannaschii

Jora

Solivio

et al. 2019

J Bacteriol

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“…Among new sequences are sets of tRNAs from two bacterial species: Streptomyces griseus and Lactococcus lactis ( 19 , 20 ), 60 and 26 sequences, respectively. As technology and methods improve, well-studied sequences continue to undergo revision ( 21 ). We have also introduced links of human tRNA sequences to MINTbase ( 22 ), which is a framework for the interactive exploration of mitochondrial and nuclear tRNA fragments.…”

Section: Database Contentmentioning

confidence: 99%

MODOMICS: a database of RNA modification pathways. 2017 update

Boccaletto

Machnicka

Purta

et al. 2017

Nucleic Acids Research

1,548

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MODOMICS is a database of RNA modifications that provides comprehensive information concerning the chemical structures of modified ribonucleosides, their biosynthetic pathways, the location of modified residues in RNA sequences, and RNA-modifying enzymes. In the current database version, we included the following new features and data: extended mass spectrometry and liquid chromatography data for modified nucleosides; links between human tRNA sequences and MINTbase - a framework for the interactive exploration of mitochondrial and nuclear tRNA fragments; new, machine-friendly system of unified abbreviations for modified nucleoside names; sets of modified tRNA sequences for two bacterial species, updated collection of mammalian tRNA modifications, 19 newly identified modified ribonucleosides and 66 functionally characterized proteins involved in RNA modification. Data from MODOMICS have been linked to the RNAcentral database of RNA sequences. MODOMICS is available at http://modomics.genesilico.pl.

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“…These phenotypes do not have immediately obvious links to ribosome function. Two of the genes deleted in the Δ⌿7 strain, rluA and rluF, encode dual-specificity enzymes responsible for ⌿ modifications in certain tRNAs as well as in rRNA (35,36). Thus, some of the phenotypes of the Δ⌿7 strain, including, perhaps, hypersensitivity to hydroxamates, may be due to altered tRNA functionality rather than to ribosome hypomodification.…”

Section: Resultsmentioning

confidence: 99%

Pseudouridine-Free Escherichia coli Ribosomes

2018

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Pseudouridine (Ψ) is present at conserved, functionally important regions in the ribosomal RNAs (rRNAs) from all three domains of life. Little, however, is known about the functions of Ψ modifications in bacterial ribosomes. An strain has been constructed in which all seven rRNA Ψ synthases have been inactivated and whose ribosomes are devoid of all Ψs. Surprisingly, this strain displays only minor defects in ribosome biogenesis and function, and cell growth is only modestly affected. This is in contrast to a strong requirement for Ψ in eukaryotic ribosomes and suggests divergent roles for rRNA Ψ modifications in these two domains. Pseudouridine (Ψ) is the most abundant posttranscriptional modification in RNAs. In the ribosome, Ψ modifications are typically located at conserved, critical regions, suggesting they play an important functional role. In eukarya and archaea, rRNAs are modified by a single pseudouridine synthase (PUS) enzyme, targeted to rRNA via a snoRNA-dependent mechanism, while bacteria use multiple stand-alone PUS enzymes. Disruption of Ψ modification of rRNA in eukarya seriously impairs ribosome function and cell growth. We have constructed an multiple deletion strain lacking all Ψ modifications in rRNA. In contrast to the equivalent eukaryotic mutants, the strain is only modestly affected in growth, decoding, and ribosome biogenesis, indicating a differential requirement for Ψ modifications in these two domains.

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Pseudouridine in the Anticodon of Escherichia coli tRNATyr(QΨA) Is Catalyzed by the Dual Specificity Enzyme RluF

Cited by 38 publications

References 61 publications

tRNA Modification Profiles and Codon-Decoding Strategies in Methanocaldococcus jannaschii

tRNA Modification Profiles and Codon-Decoding Strategies in Methanocaldococcus jannaschii

MODOMICS: a database of RNA modification pathways. 2017 update

Pseudouridine-Free Escherichia coli Ribosomes

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