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Featured researches published by Naoki Shigi.


Journal of Biological Chemistry | 2006

Identification of Two tRNA Thiolation Genes Required for Cell Growth at Extremely High Temperatures

Naoki Shigi; Yuriko Sakaguchi; Tsutomu Suzuki; Kimitsuna Watanabe

Thermostability of tRNA in thermophilic bacteria is effected by post-transcriptional modifications, such as 2-thioribothymidine (s2T) at position 54. Using a proteomics approach, we identified two genes (ttuA and ttuB; tRNA-two-thiouridine) that are essential for the synthesis of s2T in Thermus thermophilus. Mutation of either gene completely abolishes thio-modification of s2T, and these mutants exhibit a temperature-sensitive phenotype. These results suggest that bacterial growth at higher temperatures is achieved through the thermal stabilization of tRNA by a 2-thiolation modification. TtuA (TTC0106) is possibly an ATPase possessing a P-loop motif. TtuB (TTC0105) is a putative thio-carrier protein that exhibits significant sequence homology with ThiS of the thiamine synthesis pathway. Both TtuA and TtuB are required for in vitro s2T formation in the presence of cysteine and ATP. The addition of cysteine desulfurases such as IscS (TTC0087) or SufS (TTC1373) enhances the sulfur transfer reaction in vitro.


Journal of Biological Chemistry | 2002

Conserved Bases in the TΨC Loop of tRNA Are Determinants for Thermophile-specific 2-Thiouridylation at Position 54

Naoki Shigi; Tsutomu Suzuki; Masatada Tamakoshi; Tairo Oshima; Kimitsuna Watanabe

2-Thioribothymidine (s2T) is a post-transcriptionally modified nucleoside of U54 specifically found in thermophilic bacterial tRNAs. The 2-thiocarbonyl group of s2T54 is known to be responsible for the thermostability of tRNA. The s2T54 content in tRNA varies depending on the cultivation temperature, a feature that confers thermal adaptation of protein synthesis in Thermus thermophilus. Little is known about the biosynthesis of s2T, including the sulfur donor, modification enzyme, and the tRNA structural requirements. To characterize 2-thiolation at position 54 in tRNA, we constructed an in vivo expression system using tRNAAsp with an altered sequence and a host-vector for T. thermophilus. We were able to detectin vivo activity of s2T54 thiolase using phenyl mercuric gel electrophoresis followed by Northern hybridization. 2-Thiolation at position 54 was identified in the precursor form of the tRNA, indicating that 2-thiolation precedes tRNA processing. To ascertain the elements that determine 2-thiolation in tRNA, systematic site-directed mutagenesis was carried out using the tRNAAspgene. Conserved residues C56 and A58 were identified as major determinants of 2-thiolation, whereas tertiary interaction between the T and D loops and non-conserved nucleosides in the T loop were revealed not to be important for the reaction.


The EMBO Journal | 2008

Common thiolation mechanism in the biosynthesis of tRNA thiouridine and sulphur-containing cofactors.

Naoki Shigi; Yuriko Sakaguchi; Shin-ichi Asai; Tsutomu Suzuki; Kimitsuna Watanabe

2‐Thioribothymidine (s2T), a modified uridine, is found at position 54 in transfer RNAs (tRNAs) from several thermophiles; s2T stabilizes the L‐shaped structure of tRNA and is essential for growth at higher temperatures. Here, we identified an ATPase (tRNA‐two‐thiouridine C, TtuC) required for the 2‐thiolation of s2T in Thermus thermophilus and examined in vitro s2T formation by TtuC and previously identified s2T‐biosynthetic proteins (TtuA, TtuB, and cysteine desulphurases). The C‐terminal glycine of TtuB is first activated as an acyl‐adenylate by TtuC and then thiocarboxylated by cysteine desulphurases. The sulphur atom of thiocarboxylated TtuB is transferred to tRNA by TtuA. In a ttuC mutant of T. thermophilus, not only s2T, but also molybdenum cofactor and thiamin were not synthesized, suggesting that TtuC is shared among these biosynthetic pathways. Furthermore, we found that a TtuB—TtuC thioester was formed in vitro, which was similar to the ubiquitin‐E1 thioester, a key intermediate in the ubiquitin system. The results are discussed in relation to the mechanism and evolution of the eukaryotic ubiquitin system.


Frontiers in Genetics | 2014

Biosynthesis and functions of sulfur modifications in tRNA

Naoki Shigi

Sulfur is an essential element for a variety of cellular constituents in all living organisms. In tRNA molecules, there are many sulfur-containing nucleosides, such as the derivatives of 2-thiouridine (s2U), 4-thiouridine (s4U), 2-thiocytidine (s2C), and 2-methylthioadenosine (ms2A). Earlier studies established the functions of these modifications for accurate and efficient translation, including proper recognition of the codons in mRNA or stabilization of tRNA structure. In many cases, the biosynthesis of these sulfur modifications starts with cysteine desulfurases, which catalyze the generation of persulfide (an activated form of sulfur) from cysteine. Many sulfur-carrier proteins are responsible for delivering this activated sulfur to each biosynthesis pathway. Finally, specific “modification enzymes” activate target tRNAs and then incorporate sulfur atoms. Intriguingly, the biosynthesis of 2-thiouridine in all domains of life is functionally and evolutionarily related to the ubiquitin-like post-translational modification system of cellular proteins in eukaryotes. This review summarizes the recent characterization of the biosynthesis of sulfur modifications in tRNA and the novel roles of this modification in cellular functions in various model organisms, with a special emphasis on 2-thiouridine derivatives. Each biosynthesis pathway of sulfur-containing molecules is mutually modulated via sulfur trafficking, and 2-thiouridine and codon usage bias have been proposed to control the translation of specific genes.


Journal of Biological Chemistry | 2012

Posttranslational modification of cellular proteins by a ubiquitin-like protein in bacteria.

Naoki Shigi

Background: Modification of proteins by ubiquitin (Ub) and ubiquitin-like proteins (Ubls) is essential in eukaryotes. Results: Proteins for tRNA-thiouridine synthesis and other proteins are modified by a bacterial Ubl in Thermus thermophilus. Conclusion: The existence of a Ub/Ubl homologous conjugation system in Bacteria is demonstrated. Significance: This suggests an ancient origin of the eukaryotic Ub/Ubl system. Posttranslational modification of proteins with ubiquitin and ubiquitin-like proteins plays important regulatory roles in eukaryotes. Although a homologous conjugation system has recently been reported in Archaea, there is no similar report in Bacteria. This report describes the identification of a ubiquitin-like conjugation system in the bacterium Thermus thermophilus. A series of in vivo analyses revealed that TtuB, a bacterial ubiquitin-like protein that functions as a sulfur carrier in tRNA thiouridine synthesis, was covalently attached to target proteins, most likely via its C-terminal glycine. The involvement of the ubiquitin-activating enzyme-like protein TtuC in conjugate formation and the attachments of TtuB to TtuC and TtuA, which are proteins required for tRNA thiouridine synthesis, were demonstrated. Mass spectrometry analysis revealed that lysine residues (Lys-137/Lys-226/Lys-229) of TtuA were covalently modified by the C-terminal carboxylate of TtuB. Intriguingly, a deletion mutant of a JAMM (JAB1/MPN/Mov34 metalloenzyme) ubiquitin isopeptidase homolog showed aberrant TtuB conjugates of TtuC and TtuA and an ∼50% decrease in thiouridine amounts in tRNA. These results would support the hypothesis that thiouridine synthesis is regulated by TtuB-conjugation.


Journal of Biological Chemistry | 2011

Taurine-containing Uridine Modifications in tRNA Anticodons Are Required to Decipher Non-universal Genetic Codes in Ascidian Mitochondria

Takeo Suzuki; Kenjyo Miyauchi; Tsutomu Suzuki; Shin-ichi Yokobori; Naoki Shigi; Akiko Kondow; Nono Takeuchi; Akihiko Yamagishi; Kimitsuna Watanabe

Variations in the genetic code are found frequently in mitochondrial decoding systems. Four non-universal genetic codes are employed in ascidian mitochondria: AUA for Met, UGA for Trp, and AGA/AGG(AGR) for Gly. To clarify the decoding mechanism for the non-universal genetic codes, we isolated and analyzed mitochondrial tRNAs for Trp, Met, and Gly from an ascidian, Halocynthia roretzi. Mass spectrometric analysis identified 5-taurinomethyluridine (τm5U) at the anticodon wobble positions of tRNAMet(AUR), tRNATrp(UGR), and tRNAGly(AGR), suggesting that τm5U plays a critical role in the accurate deciphering of all four non-universal codes by preventing the misreading of pyrimidine-ending near-cognate codons (NNY) in their respective family boxes. Acquisition of the wobble modification appears to be a prerequisite for the genetic code alteration.


Journal of Biological Chemistry | 2015

Substrate tRNA Recognition Mechanism of Eubacterial tRNA (m1A58) Methyltransferase (TrmI)

Hiroyuki Takuma; Natsumi Ushio; Masayuki Minoji; Ai Kazayama; Naoki Shigi; Akira Hirata; Chie Tomikawa; Anna Ochi; Hiroyuki Hori

Background: tRNA methyltransferases specifically recognize substrate tRNAs. Results: To clarify the tRNA recognition mechanism of TrmI, three tRNA species and 45 variants were analyzed in vitro and in vivo. Conclusion: TrmI recognizes the aminoacyl stem, variable region, C56, purine 57, A58, and U60 in the T-loop of tRNA. Significance: Our in vitro experimental results explain the regulation of in vivo methylation levels in tRNAs. TrmI generates N1-methyladenosine at position 58 (m1A58) in tRNA. The Thermus thermophilus tRNAPhe transcript was methylated efficiently by T. thermophilus TrmI, whereas the yeast tRNAPhe transcript was poorly methylated. Fourteen chimeric tRNA transcripts derived from these two tRNAs revealed that TrmI recognized the combination of aminoacyl stem, variable region, and T-loop. This was confirmed by 10 deletion tRNA variants: TrmI methylated transcripts containing the aminoacyl stem, variable region, and T-arm. The requirement for the T-stem itself was confirmed by disrupting the T-stem. Disrupting the interaction between T- and D-arms accelerated the methylation, suggesting that this disruption is included in part of the reaction. Experiments with 17 point mutant transcripts elucidated the positive sequence determinants C56, purine 57, A58, and U60. Replacing A58 with inosine and 2-aminopurine completely abrogated methylation, demonstrating that the 6-amino group in A58 is recognized by TrmI. T. thermophilus tRNAGGUThrGGUThr contains C60 instead of U60. The tRNAGGUThr transcript was poorly methylated by TrmI, and replacing C60 with U increased the methylation, consistent with the point mutation experiments. A gel shift assay revealed that tRNAGGUThr had a low affinity for TrmI than tRNAPhe. Furthermore, analysis of tRNAGGUThr purified from the trmI gene disruptant strain revealed that the other modifications in tRNA accelerated the formation of m1A58 by TrmI. Moreover, nucleoside analysis of tRNAGGUThr from the wild-type strain indicated that less than 50% of tRNAGGUThr contained m1A58. Thus, the results from the in vitro experiments were confirmed by the in vivo methylation patterns.


Proteins | 2013

Crystallographic and mutational studies on the tRNA thiouridine synthetase TtuA.

Hirofumi Nakagawa; Mitsuo Kuratani; Sakurako Goto-Ito; Takuhiro Ito; Kazushige Katsura; Takaho Terada; Mikako Shirouzu; Shun-ichi Sekine; Naoki Shigi; Shigeyuki Yokoyama

In thermophilic bacteria, specific 2‐thiolation occurs on the conserved ribothymidine at position 54 (T54) in tRNAs, which is necessary for survival at high temperatures. T54 2‐thiolation is achieved by the tRNA thiouridine synthetase TtuA and sulfur‐carrier proteins. TtuA has five conserved CXXC/H motifs and the signature PP motif, and belongs to the TtcA family of tRNA 2‐thiolation enzymes, for which there is currently no structural information. In this study, we determined the crystal structure of a TtuA homolog from the hyperthermophilic archeon Pyrococcus horikoshii at 2.1 Å resolution. The P. horikoshii TtuA forms a homodimer, and each subunit contains a catalytic domain and unique N‐ and C‐terminal zinc fingers. The catalytic domain has much higher structural similarity to that of another tRNA modification enzyme, TilS (tRNAIle2 lysidine synthetase), than to the other type of tRNA 2‐thiolation enzyme, MnmA. Three conserved cysteine residues are clustered in the putative catalytic site, which is not present in TilS. An in vivo mutational analysis in the bacterium Thermus thermophilus demonstrated that the three conserved cysteine residues and the putative ATP‐binding residues in the catalytic domain are important for the TtuA activity. A positively charged surface that includes the catalytic site and the two zinc fingers is likely to provide the tRNA‐binding site. Proteins 2013; 81:1232–1244.


Genes to Cells | 2016

Folate-/FAD-dependent tRNA methyltransferase from Thermus thermophilus regulates other modifications in tRNA at low temperatures.

Ryota Yamagami; Chie Tomikawa; Naoki Shigi; Ai Kazayama; Shin-ichi Asai; Hiroyuki Takuma; Akira Hirata; Haruichi Asahara; Kimitsuna Watanabe; Satoko Yoshizawa; Hiroyuki Hori

TrmFO is a N5, N10‐methylenetetrahydrofolate (CH2THF)‐/FAD‐dependent tRNA methyltransferase, which synthesizes 5‐methyluridine at position 54 (m5U54) in tRNA. Thermus thermophilus is an extreme‐thermophilic eubacterium, which grows in a wide range of temperatures (50–83 °C). In T. thermophilus, modified nucleosides in tRNA and modification enzymes form a network, in which one modification regulates the degrees of other modifications and controls the flexibility of tRNA. To clarify the role of m5U54 and TrmFO in the network, we constructed the trmFO gene disruptant (∆trmFO) strain of T. thermophilus. Although this strain did not show any growth retardation at 70 °C, it showed a slow‐growth phenotype at 50 °C. Nucleoside analysis showed increase in 2′‐O‐methylguanosine at position 18 and decrease in N1‐methyladenosine at position 58 in the tRNA mixture from the ∆trmFO strain at 50 °C. These in vivo results were reproduced by in vitro experiments with purified enzymes. Thus, we concluded that the m5U54 modification have effects on the other modifications in tRNA through the network at 50 °C. 35S incorporations into proteins showed that the protein synthesis activity of ∆trmFO strain was inferior to the wild‐type strain at 50 °C, suggesting that the growth delay at 50 °C was caused by the inferior protein synthesis activity.


Proceedings of the National Academy of Sciences of the United States of America | 2017

Biochemical and structural characterization of oxygen-sensitive 2-thiouridine synthesis catalyzed by an iron-sulfur protein TtuA

Minghao Chen; Shin-ichi Asai; Shun Narai; Shusuke Nambu; Naoki Omura; Yuriko Sakaguchi; Tsutomu Suzuki; Masao Ikeda-Saito; Kimitsuna Watanabe; Min Yao; Naoki Shigi; Yoshikazu Tanaka

Significance One of the posttranscriptional modifications of tRNA, 2-thiouridine (s2U), enhances thermostability. Although extensive studies have been conducted to understand the mechanism behind this modification, many ill-defined points remain, because the S-transfer enzyme 2-thiouridine synthetase TtuA has shown very low activity in previous in vitro experiments. Here we demonstrate that TtuA requires oxygen-labile [4Fe-4S] clusters for its activity. Furthermore, we determine the crystal structure of TtuA in complex with the Fe-S cluster and ATP analog and also with its S-donor protein, 2-thiouridine synthesis sulfur carrier protein (TtuB). The combined actions of TtuA and TtuB using the Fe-S cluster aid the S-transfer mechanism. Two-thiouridine (s2U) at position 54 of transfer RNA (tRNA) is a posttranscriptional modification that enables thermophilic bacteria to survive in high-temperature environments. s2U is produced by the combined action of two proteins, 2-thiouridine synthetase TtuA and 2-thiouridine synthesis sulfur carrier protein TtuB, which act as a sulfur (S) transfer enzyme and a ubiquitin-like S donor, respectively. Despite the accumulation of biochemical data in vivo, the enzymatic activity by TtuA/TtuB has rarely been observed in vitro, which has hindered examination of the molecular mechanism of S transfer. Here we demonstrate by spectroscopic, biochemical, and crystal structure analyses that TtuA requires oxygen-labile [4Fe-4S]-type iron (Fe)-S clusters for its enzymatic activity, which explains the previously observed inactivation of this enzyme in vitro. The [4Fe-4S] cluster was coordinated by three highly conserved cysteine residues, and one of the Fe atoms was exposed to the active site. Furthermore, the crystal structure of the TtuA-TtuB complex was determined at a resolution of 2.5 Å, which clearly shows the S transfer of TtuB to tRNA using its C-terminal thiocarboxylate group. The active site of TtuA is connected to the outside by two channels, one occupied by TtuB and the other used for tRNA binding. Based on these observations, we propose a molecular mechanism of S transfer by TtuA using the ubiquitin-like S donor and the [4Fe-4S] cluster.

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Akiko Nishimura

National Institute of Genetics

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Jun-ichi Kato

Tokyo Metropolitan University

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