Effect of G-1 on histidine tRNA microhelix conformation

doi:10.1093/nar/gkg930

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Nucleic Acids Research, 2003, Vol. 31, No. 24 7311-7321
© 2003 Oxford University Press

Article

Effect of G-1 on histidine tRNA microhelix conformation

Mahadevan Seetharaman¹^,2, Caroline Williams¹, Christopher J. Cramer¹^,2 and Karin Musier-Forsyth^*^,1^,2

¹ Department of Chemistry, University of Minnesota, 207 Pleasant Street S.E. and ² Minnesota Supercomputing Institute, University of Minnesota, 117 Pleasant Street S.E., Minneapolis, MN 55455–0421, USA

*To whom correspondence should be addressed. Tel: +1 612 624 0286; Fax: 612 626 7541; Email: musier{at}chem.umn.edu
Present address:
C. Williams, Chemical Diversity Labs, San Diego, CA 92121, USA
The authors wish it to be known that, in their opinion, the first two authors should be regarded as joint First Authors

Histidine tRNAs (tRNA^His) are unique in that they possess anextra 5'-base (G-1) not found in other tRNAs. Deletion of G-1results in at least a 250-fold reduction in the rate of histidinecharging in vitro. To better understand the role of the G-1nucleotide in defining the structure of tRNA^His, and to correlatestructure with cognate amino acid charging, NMR and moleculardynamics (MD) studies were performed on the wild-type and a ${Delta}$ G-1 mutant Escherichia coli histidine tRNA acceptor stem microhelix.Using NMR-derived distance restraints, global structural characteristicsare described and interpreted to rationalize experimental observationswith respect to aminoacylation activity. The quality of theNMR-derived solution conformations of the wild-type and ${Delta}$ G-1histidine microhelices (micro helix^His) is assessed using avariety of MD-based computational protocols. Most of the duplexregions of the acceptor stem and the UUCG tetraloop are welldefined and effectively superimposable for the wild-type and ${Delta}$ G-1 mutant microhelix^His. Differences, however, are observedat the end of the helix and in the single-stranded CCCA-3' tail.The wild-type microhelix^His structure is more well defined thanthe mutant and folds into a ‘stacked fold-back’conformation. In contrast, we observe fraying of the first twobase pairs and looping back of the single-stranded region inthe ${Delta}$ G-1 mutant resulting in a much less well defined conformation.Thus the role of the extra G-1 base of the unique G-1:C73 basepair in tRNA^His may be to prevent end-fraying and stabilizethe stacked fold-back conformation of the CCCA-3' region.

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