TY - JOUR T1 - Antibody with Infinite Affinity for In Vivo Tracking of Genetically Engineered Lymphocytes JF - Journal of Nuclear Medicine JO - J Nucl Med SP - 1894 LP - 1900 DO - 10.2967/jnumed.118.208041 VL - 59 IS - 12 AU - Simone Krebs AU - Afruja Ahad AU - Lukas M. Carter AU - Justin Eyquem AU - Christian Brand AU - Meghan Bell AU - Vladimir Ponomarev AU - Thomas Reiner AU - Claude F. Meares AU - Stephen Gottschalk AU - Michel Sadelain AU - Steven M. Larson AU - Wolfgang A. Weber Y1 - 2018/12/01 UR - http://jnm.snmjournals.org/content/59/12/1894.abstract N2 - There remains an urgent need for the noninvasive tracking of transfused chimeric antigen receptor (CAR) T cells to determine their biodistribution, viability, expansion, and antitumor functionality. DOTA antibody reporter 1 (DAbR1) comprises a single-chain fragment of the antilanthanoid-DOTA antibody 2D12.5/G54C fused to the human CD4-transmembrane domain and binds irreversibly to lanthanoid (S)-2-(4-acrylamidobenzyl)-DOTA (AABD). The aim of this study was to investigate whether DAbR1 can be expressed on lymphocytes and used as a reporter gene as well as a suicide gene for therapy of immune-related adverse effects. Methods: DAbR1 was subcloned together with green fluorescent protein into an SFG-retroviral vector and used to transduce CD3/CD28-activated primary human T cells and second-generation 1928z (CAR) T cells. Cell surface expression of DAbR1 was confirmed by cell uptake studies with radiolabeled AABD. In addition, the feasibility of imaging of DAbR1-positive T cells in vivo after intravenous injection of 86Y/177Lu-AABD was studied and radiation doses determined. Results: A panel of DAbR1-expressing T cells and CAR T cells exhibited greater than 8-fold increased uptake of 86Y-AABD in vitro when compared with nontransduced cells. Imaging studies showed 86Y-AABD was retained by DAbR1-positive T cells while it continuously cleared from normal tissues, allowing for in vivo tracking of intravenously administered CAR T cells. Normal-organ dose estimates were favorable for repeated PET/CT studies. Selective T cell ablation in vivo with 177Lu-AABD seems feasible for clustered T-cell populations. Conclusion: We have demonstrated for the first time that T cells can be modified with DAbR1, enabling their in vivo tracking via PET and SPECT. The favorable biodistribution and high image contrast observed warrant further studies of this new reporter gene. ER -