Seryl-tRNA synthetase promotes translational readthrough by mRNA binding and involvement of the selenocysteine incorporation machinery

  • Ze Liu
  • , Justin Wang
  • , Yi Shi
  • , Brian A. Yee
  • , Markus Terrey
  • , Qian Zhang
  • , Jenq Chang Lee
  • , Kuo I. Lin
  • , Andrew H.J. Wang
  • , Susan L. Ackerman
  • , Gene W. Yeo
  • , Haissi Cui
  • , Xiang Lei Yang

Research output: Contribution to journalArticlepeer-review

11 Citations (Scopus)

Abstract

Translational readthrough of UGA stop codons by selenocysteine-specific tRNA (tRNASec) enables the synthesis of selenoproteins. Seryl-tRNA synthetase (SerRS) charges tRNASec with serine, which is modified into selenocysteine and delivered to the ribosome by a designated elongation factor (eEFSec in eukaryotes). Here we found that components of the human selenocysteine incorporation machinery (SerRS, tRNASec, and eEFSec) also increased translational readthrough of non-selenocysteine genes, including VEGFA, to create C-terminally extended isoforms. SerRS recognizes target mRNAs through a stem-loop structure that resembles the variable loop of its cognate tRNAs. This function of SerRS depends on both its enzymatic activity and a vertebrate-specific domain. Through eCLIP-seq, we identified additional SerRS-interacting mRNAs as potential readthrough genes. Moreover, SerRS overexpression was sufficient to reverse premature termination caused by a pathogenic nonsense mutation. Our findings expand the repertoire of selenoprotein biosynthesis machinery and suggest an avenue for therapeutic targeting of nonsense mutations using endogenous factors.

Original languageEnglish
Pages (from-to)10768-10781
Number of pages14
JournalNucleic Acids Research
Volume51
Issue number19
DOIs
Publication statusPublished - Oct 27 2023

ASJC Scopus subject areas

  • Genetics

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