Wiedemann, GertrudGertrudWiedemannBacher, UlrikeUlrikeBacherJoncourt, RaphaelRaphaelJoncourtSolly, FrançoiseFrançoiseSollyWidmer, Corinne CCorinne CWidmerZeerleder, SachaSachaZeerlederNovak, UrbanUrbanNovakPabst, ThomasThomasPabstPorret, Naomi ANaomi APorret2024-10-082024-10-082024-08-06https://boris-portal.unibe.ch/handle/20.500.12422/44732In this study, we present the design, implementation, and successful use of digital droplet PCR (ddPCR) for the monitoring of chimeric antigen receptor T-cell (CAR-T) expansion in patients with B-cell malignancies treated with different CAR-T products at our clinical center. Initially, we designed a specific and highly sensitive ddPCR assay targeting the junction between the 4-1BB and CD3ζ domains of tisa-cel, normalized with , and validated it using blood samples from the first tisa-cel-treated patient in Switzerland. We further compared this assay with a published qPCR (quantitative real-time PCR) design. Both assays showed reliable quantification of CAR-T copies down to 20 copies/µg DNA. The reproducibility and precision were confirmed through extensive testing and inter-laboratory comparisons. With the introduction of other CAR-T products, we also developed a corresponding ddPCR assay targeting axi-cel and brexu-cel, demonstrating high specificity and sensitivity with a limit of detection of 20 copies/µg DNA. These assays are suitable for CAR-T copy number quantification across multiple sample types, including peripheral blood, bone marrow, and lymph node biopsy material, showing robust performance and indicating the presence of CAR-T cells not only in the blood but also in target tissues. Longitudinal monitoring of CAR-T cell kinetics in 141 patients treated with tisa-cel, axi-cel, or brexu-cel revealed significant expansion and long-term persistence. Peak expansion correlated with clinical outcomes and adverse effects, as is now well known. Additionally, we quantified the CAR-T mRNA expression, showing a high correlation with DNA copy numbers and confirming active transgene expression. Our results highlight the quality of ddPCR for CAR-T monitoring, providing a sensitive, precise, and reproducible method suitable for clinical applications. This approach can be adapted for future CAR-T products and will support the monitoring and the management of CAR-T cell therapies.enB-cell lymphomaCAR-T cell therapiesacute lymphatic leukemia (ALL)droplet digital PCR (ddPCR)molecular monitoring600 - Technology::610 - Medicine & healtharticle10.48620/84253920124210.3390/ijms25168556