A Preliminary Study of PSMA Fluorescent Probe for Targeted Fluorescence Imaging of Prostate Cancer

Haoxi Zhou; Yachao Liu; Xiaojun Zhang; Kuang Chen; Yuan Li; Xiaodan Xu; Baixuan Xu

doi:10.3390/molecules27092736

A Preliminary Study of PSMA Fluorescent Probe for Targeted Fluorescence Imaging of Prostate Cancer

Molecules. 2022 Apr 24;27(9):2736. doi: 10.3390/molecules27092736.

Authors

Haoxi Zhou^{1

2}, Yachao Liu², Xiaojun Zhang², Kuang Chen¹, Yuan Li³, Xiaodan Xu², Baixuan Xu^{1

2}

Affiliations

¹ Chinese PLA Medical School, Chinese PLA General Hospital, Beijing 100853, China.
² Department of Nuclear Medicine, Chinese PLA General Hospital, Beijing 100853, China.
³ Department of Nuclear Medicine, Peking University First Hospital, Beijing 100034, China.

Abstract

Purpose: With the increasing detection rate of early prostate cancer (PCa), the proportion of surgical treatment is increasing. Surgery is the most effective treatment for PCa. Precise targeting of tumors during surgery can reduce the incidence of positive surgical margins (PSMs) and preserve the neurovascular bundles (NVBs) as much as possible. The objective of this study was to synthesize a PSMA fluorescent probe (PSMA-Cy5) and verify the targeting specificity of the probe for prostate cancer, thereby providing a theoretical basis for the development of PSMA fluorescent probes for clinical application in the future. Methods: In this study, a novel water-soluble 3H-indocyanine-type bioluminescent dye-Cy5-labeled prostate-specific membrane antigen (PSMA) ligand (PSMA-Cy5) was synthesized by liquid phase synthesis. The PSMA ligand was developed based on the glutamine-urea-lysine (Glu-urea-Lys) structure. The new fluorescent probe was evaluated in vitro and in vivo, and its safety was evaluated. Confocal microscopy was used to observe the binding uptake of PSMA-Cy5 with PSMA (+) LNCaP cells, PSMA (-) PC3 cells and blocked LNCaP cells. In in vivo optical imaging studies, the targeting specificity of PSMA (+) 22Rv1 tumors to probe binding was validated by tail vein injection of PSMA-Cy5. The safety of the PSMA-Cy5 probe was evaluated by histopathological analysis of mouse organs by a single high-dose tail vein injection of PSMA-Cy5. Results: In vitro fluorescence cell uptake experiments showed that the binding of PSMA-Cy5 to LNCaP cells has targeting specificity. PC3 cells and blocked LNCaP cells showed almost no uptake. The results of in vivo optical imaging studies showed that the tumor-to-background ratio in the 22Rv1 group was 3.39 ± 0.47; in the 22Rv1 blocking group it was 0.78 ± 0.15, and in the PC3 group it was 0.94 ± 0.09, consistent with the in vitro results. After a high-dose injection of PSMA-Cy5, there were no abnormalities in the tissues or organs of the mice. The probe showed good safety. Conclusions: PSMA-Cy5 is a probe with good targeting specificity and low toxicity that can accurately visualize tumors in vivo. This study has an important reference value for the development of PSMA fluorescent probes. In the future, it can be applied to precise tumor imaging during radical prostatectomy to reduce the incidence of postoperative PSM.

Keywords: PSMA; fluorescence imaging; positive surgical margin (PSM); radical prostatectomy.

MeSH terms

Animals
Antigens, Surface / metabolism
Cell Line, Tumor
Fluorescent Dyes*
Humans
Ligands
Male
Mice
Optical Imaging / methods
Prostatic Neoplasms* / metabolism
Urea

Substances

Antigens, Surface
Fluorescent Dyes
Ligands
Urea