Nature Communications (Feb 2024)

Compromised transcription-mRNA export factor THOC2 causes R-loop accumulation, DNA damage and adverse neurodevelopment

  • Rudrarup Bhattacharjee,
  • Lachlan A. Jolly,
  • Mark A. Corbett,
  • Ing Chee Wee,
  • Sushma R. Rao,
  • Alison E. Gardner,
  • Tarin Ritchie,
  • Eline J. H. van Hugte,
  • Ummi Ciptasari,
  • Sandra Piltz,
  • Jacqueline E. Noll,
  • Nazzmer Nazri,
  • Clare L. van Eyk,
  • Melissa White,
  • Dani Fornarino,
  • Cathryn Poulton,
  • Gareth Baynam,
  • Lyndsey E. Collins-Praino,
  • Marten F. Snel,
  • Nael Nadif Kasri,
  • Kim M. Hemsley,
  • Paul Q. Thomas,
  • Raman Kumar,
  • Jozef Gecz

DOI
https://doi.org/10.1038/s41467-024-45121-5
Journal volume & issue
Vol. 15, no. 1
pp. 1 – 25

Abstract

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Abstract We implicated the X-chromosome THOC2 gene, which encodes the largest subunit of the highly-conserved TREX (Transcription-Export) complex, in a clinically complex neurodevelopmental disorder with intellectual disability as the core phenotype. To study the molecular pathology of this essential eukaryotic gene, we generated a mouse model based on a hypomorphic Thoc2 exon 37–38 deletion variant of a patient with ID, speech delay, hypotonia, and microcephaly. The Thoc2 exon 37–38 deletion male (Thoc2 Δ/Y ) mice recapitulate the core phenotypes of THOC2 syndrome including smaller size and weight, and significant deficits in spatial learning, working memory and sensorimotor functions. The Thoc2 Δ/Y mouse brain development is significantly impacted by compromised THOC2/TREX function resulting in R-loop accumulation, DNA damage and consequent cell death. Overall, we suggest that perturbed R-loop homeostasis, in stem cells and/or differentiated cells in mice and the patient, and DNA damage-associated functional alterations are at the root of THOC2 syndrome.