Structural and biochemical analysis of the dual-specificity Trm10 enzyme from Thermococcus kodakaraensis prompts reconsideration of its catalytic mechanism
- Ranjan Kumar Singh1,2,6,
- André Feller3,6,
- Martine Roovers4,6,
- Dany Van Elder3,
- Lina Wauters1,2,5,
- Louis Droogmans3 and
- Wim Versées1,2
- 1Structural Biology Brussels, Vrije Universiteit Brussel, 1050 Brussels, Belgium
- 2VIB-VUB Center For Structural Biology, 1050 Brussels, Belgium
- 3Laboratoire de Microbiologie, Université libre de Bruxelles (ULB), 6041 Gosselies, Belgium
- 4Institut de Recherches Microbiologiques Jean-Marie Wiame - Labiris, 1070 Brussels, Belgium
- 5Department of Cell Biochemistry, University of Groningen, Groningen 9747 AG, Netherlands
- Corresponding authors: wim.versees{at}vub.be, ldroogma{at}ulb.ac.be
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↵6 These authors contributed equally to this work.
Abstract
tRNA molecules get heavily modified post-transcriptionally. The N-1 methylation of purines at position 9 of eukaryal and archaeal tRNA is catalyzed by the SPOUT methyltranferase Trm10. Remarkably, while certain Trm10 orthologs are specific for either guanosine or adenosine, others show a dual specificity. Structural and functional studies have been performed on guanosine- and adenosine-specific enzymes. Here we report the structure and biochemical analysis of the dual-specificity enzyme from Thermococcus kodakaraensis (TkTrm10). We report the first crystal structure of a construct of this enzyme, consisting of the N-terminal domain and the catalytic SPOUT domain. Moreover, crystal structures of the SPOUT domain, either in the apo form or bound to S-adenosyl-l-methionine or S-adenosyl-l-homocysteine reveal the conformational plasticity of two active site loops upon substrate binding. Kinetic analysis shows that TkTrm10 has a high affinity for its tRNA substrates, while the enzyme on its own has a very low methyltransferase activity. Mutation of either of two active site aspartate residues (Asp206 and Asp245) to Asn or Ala results in only modest effects on the N-1 methylation reaction, with a small shift toward a preference for m1G formation over m1A formation. Only a double D206A/D245A mutation severely impairs activity. These results are in line with the recent finding that the single active-site aspartate was dispensable for activity in the guanosine-specific Trm10 from yeast, and suggest that also dual-specificity Trm10 orthologs use a noncanonical tRNA methyltransferase mechanism without residues acting as general base catalysts.
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Article is online at http://www.rnajournal.org/cgi/doi/10.1261/rna.064345.117.
- Received October 3, 2017.
- Accepted May 21, 2018.
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