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Copy number variation in tRNA isodecoder genes impairs mammalian development and balanced translation

Author

Listed:
  • Laetitia A. Hughes

    (Harry Perkins Institute of Medical Research
    QEII Medical Centre
    The University of Western Australia, QEII Medical Centre)

  • Danielle L. Rudler

    (Harry Perkins Institute of Medical Research
    QEII Medical Centre
    The University of Western Australia, QEII Medical Centre)

  • Stefan J. Siira

    (Harry Perkins Institute of Medical Research
    QEII Medical Centre
    The University of Western Australia, QEII Medical Centre)

  • Tim McCubbin

    (The University of Queensland)

  • Samuel A. Raven

    (Harry Perkins Institute of Medical Research
    QEII Medical Centre
    The University of Western Australia, QEII Medical Centre)

  • Jasmin M. Browne

    (Harry Perkins Institute of Medical Research
    QEII Medical Centre
    The University of Western Australia, QEII Medical Centre)

  • Judith A. Ermer

    (Harry Perkins Institute of Medical Research
    QEII Medical Centre
    The University of Western Australia, QEII Medical Centre)

  • Jeanette Rientjes

    (Monash University)

  • Jennifer Rodger

    (The University of Western Australia
    Perron Institute for Neurological and Translational Sciences)

  • Esteban Marcellin

    (QEII Medical Centre
    The University of Queensland
    The University of Queensland)

  • Oliver Rackham

    (Harry Perkins Institute of Medical Research
    QEII Medical Centre
    Curtin University
    Curtin University)

  • Aleksandra Filipovska

    (Harry Perkins Institute of Medical Research
    QEII Medical Centre
    The University of Western Australia, QEII Medical Centre
    Perth Children’s Hospital)

Abstract

The number of tRNA isodecoders has increased dramatically in mammals, but the specific molecular and physiological reasons for this expansion remain elusive. To address this fundamental question we used CRISPR editing to knockout the seven-membered phenylalanine tRNA gene family in mice, both individually and combinatorially. Using ATAC-Seq, RNA-seq, ribo-profiling and proteomics we observed distinct molecular consequences of single tRNA deletions. We show that tRNA-Phe-1-1 is required for neuronal function and its loss is partially compensated by increased expression of other tRNAs but results in mistranslation. In contrast, the other tRNA-Phe isodecoder genes buffer the loss of each of the remaining six tRNA-Phe genes. In the tRNA-Phe gene family, the expression of at least six tRNA-Phe alleles is required for embryonic viability and tRNA-Phe-1-1 is most important for development and survival. Our results reveal that the multi-copy configuration of tRNA genes is required to buffer translation and viability in mammals.

Suggested Citation

  • Laetitia A. Hughes & Danielle L. Rudler & Stefan J. Siira & Tim McCubbin & Samuel A. Raven & Jasmin M. Browne & Judith A. Ermer & Jeanette Rientjes & Jennifer Rodger & Esteban Marcellin & Oliver Rackh, 2023. "Copy number variation in tRNA isodecoder genes impairs mammalian development and balanced translation," Nature Communications, Nature, vol. 14(1), pages 1-19, December.
  • Handle: RePEc:nat:natcom:v:14:y:2023:i:1:d:10.1038_s41467-023-37843-9
    DOI: 10.1038/s41467-023-37843-9
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    2. Fran Supek & Matko Bošnjak & Nives Škunca & Tomislav Šmuc, 2011. "REVIGO Summarizes and Visualizes Long Lists of Gene Ontology Terms," PLOS ONE, Public Library of Science, vol. 6(7), pages 1-9, July.
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