Synthesis and preclinical evaluation of novel 18F-labeled Glu-urea-Glu-based PSMA inhibitors for prostate cancer imaging: a comparison with 18F-DCFPyl and 18F-PSMA-1007

Stephanie Robu; Alexander Schmidt; Matthias Eiber; Margret Schottelius; Thomas Günther; Behrooz Hooshyar Yousefi; Markus Schwaiger; Hans-Jürgen Wester

doi:10.1186/s13550-018-0382-8

Synthesis and preclinical evaluation of novel ¹⁸F-labeled Glu-urea-Glu-based PSMA inhibitors for prostate cancer imaging: a comparison with ¹⁸F-DCFPyl and ¹⁸F-PSMA-1007

EJNMMI Res. 2018 Apr 12;8(1):30. doi: 10.1186/s13550-018-0382-8.

Authors

Stephanie Robu¹, Alexander Schmidt², Matthias Eiber³, Margret Schottelius², Thomas Günther², Behrooz Hooshyar Yousefi³, Markus Schwaiger³, Hans-Jürgen Wester²

Affiliations

¹ Chair of Pharmaceutical Radiochemistry, Technical University Munich, Walther-Meissner-Strasse 3, 85748, Garching, Germany. stephanie.robu@tum.de.
² Chair of Pharmaceutical Radiochemistry, Technical University Munich, Walther-Meissner-Strasse 3, 85748, Garching, Germany.
³ Department of Nuclear Medicine, Klinikum rechts der Isar, Technical University Munich, Ismaningerstr. 22, 81675, Munich, Germany.

Abstract

Background: Due to its high and consistent expression in prostate cancer (PCa), the prostate-specific membrane antigen (PSMA) represents an ideal target for molecular imaging and targeted therapy using highly specific radiolabeled PSMA ligands. To address the continuously growing clinical demand for ¹⁸F-labeled PSMA-probes, we developed two novel Glu-urea-Glu-(EuE)-based inhibitors, EuE-k-¹⁸F-FBOA (1) and EuE-k-β-a-¹⁸F-FPyl (2), both with optimized linker structure and different ¹⁸F-labeled aromatic moieties. The inhibitors were evaluated in a comparative preclinical study with ¹⁸F-DCFPyl and ¹⁸F-PSMA-1007.

Results: Radiolabeling procedures allowed preparation of (1) and (2) with high radiochemical yields (67 ± 7 and 53 ± 7%, d.c.) and purity (> 98%). When compared with ¹⁸F-DCFPyl (IC₅₀ = 12.3 ± 1.2 nM) and ¹⁸F-PSMA-1007 (IC₅₀ = 4.2 ± 0.5 nM), both metabolically stable EuE-based ligands showed commensurable or higher PSMA affinity (IC₅₀ = 4.2 ± 0.4 nM (1), IC₅₀ = 1.1 ± 0.2 nM (2)). Moreover, 1.4- and 2.7-fold higher internalization rates were observed for (1) and (2), respectively, resulting in markedly enhanced tumor accumulation in LNCaP-tumor-bearing mice ((1) 12.7 ± 2.0% IA/g, (2) 13.0° ± 1.0% IA/g vs. 7.3 ± 1.0% IA/g (¹⁸F-DCFPyl), 7.1 ± 1.5% IA/g (¹⁸F-PSMA-1007), 1 h p.i.). In contrast to (1), (2) showed higher kidney accumulation and delayed clearance kinetics. Due to the high hydrophilicity of both compounds, almost no unspecific uptake in non-target tissue was observed. In contrast, due to the less hydrophilic character (logP = - 1.6) and high plasma protein binding (98%), ¹⁸F-PSMA-1007 showed uptake in non-target tissue and predominantly hepatobiliary excretion, whereas, ¹⁸F-DCFPyl exhibited pharmacokinetics quite similar to those obtained with (1) and (2).

Conclusion: Both ¹⁸F-labeled EuE-based PSMA ligands showed excellent in vitro and in vivo PSMA-targeting characteristics. The substantially higher tumor accumulation in mice compared to recently introduced ¹⁸F-PSMA-1007 and ¹⁸F-DCFPyl suggests their high value for preclinical studies investigating the effects on PSMA-expression. In contrast to (2), (1) seems to be more promising for further investigation, due to the more reliable ¹⁸F-labeling procedure, the faster clearance kinetics with comparable high tumor uptake, resulting therefore in better high-contrast microPET imaging as early as 1 h p.i.

Keywords: 18F-DCFPyl; 18F-PSMA-1007; 18F-labeled EuE-based inhibitors; PET prostate Cancer imaging; PSMA.

Grants and funding

SFB824, subproject B11, Z1/Deutsche Forschungsgemeinschaft