CAR T cell manufacturing from naive/stem memory T lymphocytes enhances antitumor responses while curtailing cytokine release syndrome
Silvia Arcangeli, … , Attilio Bondanza, Monica Casucci
Silvia Arcangeli, … , Attilio Bondanza, Monica Casucci
Published May 3, 2022
Citation Information: J Clin Invest. 2022;132(12):e150807. https://doi.org/10.1172/JCI150807.
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Research Article Immunology

CAR T cell manufacturing from naive/stem memory T lymphocytes enhances antitumor responses while curtailing cytokine release syndrome

Abstract

Chimeric antigen receptor (CAR) T cell expansion and persistence represent key factors to achieve complete responses and prevent relapses. These features are typical of early memory T cells, which can be highly enriched through optimized manufacturing protocols. Here, we investigated the efficacy and safety profiles of CAR T cell products generated from preselected naive/stem memory T cells (TN/SCM), as compared with unselected T cells (TBULK). Notwithstanding their reduced effector signature in vitro, limiting CAR TN/SCM doses showed superior antitumor activity and the unique ability to counteract leukemia rechallenge in hematopoietic stem/precursor cell–humanized mice, featuring increased expansion rates and persistence together with an ameliorated exhaustion and memory phenotype. Most relevantly, CAR TN/SCM proved to be intrinsically less prone to inducing severe cytokine release syndrome, independently of the costimulatory endodomain employed. This safer profile was associated with milder T cell activation, which translated into reduced monocyte activation and cytokine release. These data suggest that CAR TN/SCM are endowed with a wider therapeutic index compared with CAR TBULK.

Authors

Silvia Arcangeli, Camilla Bove, Claudia Mezzanotte, Barbara Camisa, Laura Falcone, Francesco Manfredi, Eugenia Bezzecchi, Rita El Khoury, Rossana Norata, Francesca Sanvito, Maurilio Ponzoni, Beatrice Greco, Marta Angiola Moresco, Matteo G. Carrabba, Fabio Ciceri, Chiara Bonini, Attilio Bondanza, Monica Casucci

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Figure 7

CAR TN/SCM can be generated from patients with B-ALL.

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CAR TN/SCM can be generated from patients with B-ALL. CD62L+CD45RA+ doub...
CD62L+CD45RA+ double-positive T cells from patients with B-ALL were isolated by FACS and bulk unselected T cells were employed as control. TN/SCM and TBULK were activated with TransAct, transduced with lentiviral vector encoding either a CD19.28z CAR or a CD19.BBz CAR, and expanded in culture with IL-7 and IL-15. (A) T cell fold expansion at the end of culture protocol (CAR TBULK/CAR TN/SCM 28z n = 3, CAR TBULK/CAR TN/SCM BBz n = 3). (B) TSCM enrichment, (C) CD8+ frequency, and (D) HLA-DR expression at the end of manufacturing. (E) T cell proliferation after a 4-day coculture with NALM-6 cells, measured by intracellular staining of Ki-67. (F) Killing activity expressed as elimination index (see Methods) and measured by coculturing CAR T cells with NALM-6, BV173, and ALL-CM CD19+ tumor cells for 4 days at a 1:20 effector/target (E:T) ratio (CAR TBULK/CAR TN/SCM 28z n = 9, CAR TBULK/CAR TN/SCM BBz n = 6). (G) Cytokine (CTK) production after 24-hour coculture of CAR T cells with CD19+ cell lines at a 1:10 E:T ratio. Full circles refer to CAR constructs carrying the CD28 costimulatory domain, while open circles refer to CAR constructs carrying 4-1BB. Data are represented as mean ± SEM together with overlapping scattered values. *P < 0.05 by paired t test.