• The ATO supports healthy HSPC differentiation into polyclonal αβ/γδ T cells; RAG1-SCID HSPCs arrest at CD4+/CD8dim stage without TCRs.

  • Lentiviral gene addition of RAG1 results in correction of the developmental block and a polyclonal αβ and γδ T cell repertoire.

Recombination activating gene 1 (RAG1) is essential for V(D)J recombination during early T and B cell development. Null mutations cause a complete block in receptor rearrangement, resulting in T⁻B⁻ severe combined immunodeficiency (SCID). Patients with RAG1-SCID require hematopoietic stem cell transplantation for survival. Our phase I/II clinical trial (NCT04797260) is currently evaluating lentiviral RAG1 gene addition in autologous hematopoietic stem and progenitor cells (HSPCs). However, studying early human T cell development is challenging due to limited access to thymic tissue. The artificial thymic organoid (ATO) system offers a promising in vitro model to study human T cell differentiation. Here, we show that ATO cultures efficiently support T cell development from healthy donor HSPCs derived from umbilical cord blood (UCB) or mobilized peripheral blood (mPB), yielding not only αβ but also γδ T cells with a polyclonal T cell receptor (TCR) repertoire. In contrast, non-corrected RAG1-deficient HSPCs from three RAG1-SCID patients show a developmental arrest before or at the aberrant CD4⁺CD8dim double-positive stage, characterized by minimal or absent CD1a upregulation and CD7 downregulation, absence of TCRβ (TRB) rearrangement, and only partial TCRγ (TRG) and TCRδ (TRD) rearrangement. Lentiviral RAG1 gene addition using the clinical vector rescues T cell development in these patient-derived HSPCs and restores TCR repertoire diversity. These findings highlight the ATO system as a valuable model for dissecting human T cell development and for the preclinical development and evaluation of gene therapy.

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First page of RAG1 lentiviral gene therapy restores T cell development of RAG1-SCID patient cells in artificial thymic organoids

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