4.6 Article

Importance of a tRNA anticodon loop modification and a conserved, noncanonical anticodon stem pairing in tRNACGGPro for decoding

期刊

JOURNAL OF BIOLOGICAL CHEMISTRY
卷 294, 期 14, 页码 5281-5291

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ELSEVIER
DOI: 10.1074/jbc.RA119.007410

关键词

translation; ribosome; transfer RNA (tRNA); RNA modification; mRNA; structural biology; decoding; mRNA frame maintenance

资金

  1. NIGMS, National Institutes of Health [P30 GM124165]
  2. National Institutes of Health [RR25528, RR028976]
  3. APS, a United States Department of Energy Office of Science User Facility [DE-AC02-06CH11357, W-31-109-Eng-38]

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Modification of anticodon nucleotides allows tRNAs to decode multiple codons, expanding the genetic code. Additionally, modifications located in the anticodon loop, but outside the anticodon itself, stabilize tRNA-codon interactions, increasing decoding fidelity. Anticodon loop nucleotide 37 is 3 to the anticodon and, in tRNAPro, is methylated at the N1 position in its nucleobase (m(1)G37). The m(1)G37 modification in tRNAPro stabilizes its interaction with the codon and maintains the mRNA frame. However, it is unclear how m(1)G37 affects binding at the decoding center to both cognate and +1 slippery codons. Here, we show that the tRNAPro m(1)G37 modification is important for the association step during binding to a cognate CCG codon. In contrast, m(1)G37 prevented association with a slippery CCC-U or +1 codon. Similar analyses of frameshift suppressor tRNA(SufA6), a tRNAPro derivative containing an extra nucleotide in its anticodon loop that undergoes +1 frameshifting, reveal that m(1)G37 destabilizes interactions with both the cognate CCG and slippery codons. One reason for this destabilization is the disruption of a conserved U32A38 nucleotide pairing in the anticodon stem through insertion of G37.5. Restoring the tRNA(SufA6) U32A37.5 pairing results in a high-affinity association on the slippery CCC-U codon. Further, an X-ray crystal structure of the 70S ribosome bound to tRNA(SufA6) U32A37.5 at 3.6 angstrom resolution shows a reordering of the anticodon loop consistent with the findings from the high-affinity measurements. Our results reveal how the tRNA modification at nucleotide 37 stabilizes interactions with the mRNA codon to preserve the mRNA frame.

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