99mTc-Labeled Cyclic Peptide Targeting PD-L1 as a Novel Nuclear Imaging Probe

Guillermina Ferro-Flores; Blanca Ocampo-García; Pedro Cruz-Nova; Myrna Luna-Gutiérrez; Gerardo Bravo-Villegas; Erika Azorín-Vega; Nallely Jiménez-Mancilla; Emiliano Michel-Sánchez; Osvaldo García-Pérez; Nancy Lara-Almazán; Clara Santos-Cuevas

doi:10.3390/pharmaceutics15122662

^99mTc-Labeled Cyclic Peptide Targeting PD-L1 as a Novel Nuclear Imaging Probe

Pharmaceutics. 2023 Nov 23;15(12):2662. doi: 10.3390/pharmaceutics15122662.

Affiliations

¹ Department of Radioactive Materials, Instituto Nacional de Investigaciones Nucleares, Ocoyoacac 52750, Mexico.
² Faculty of Chemistry, Universidad Autónoma del Estado de México, Toluca 50180, Mexico.
³ Cátedras, CONACyT, Instituto Nacional de Investigaciones Nucleares, Ocoyoacac 52750, Mexico.
⁴ Department of Nuclear Medicine, Instituto Nacional de Cancerología, Tlalpan, Mexico City 14080, Mexico.

Abstract

Recent cancer therapies have focused on reducing immune suppression in the tumor microenvironment to prevent cancer progression and metastasis. PD-1 is a checkpoint protein that stops the immune response and is expressed on immune T cells. Cancer cells express a PD-1 ligand (PD-L1) to bind to the T-cell surface and activate immunosuppressive pathways. This study aimed to design, synthesize, and evaluate a ^99mTc-labeled PD-L1-targeting cyclic peptide inhibitor (^99mTc-iPD-L1) as a novel SPECT radiopharmaceutical for PD-L1 expression imaging. AutoDock software (version 1.5) was used to perform molecular docking for affinity calculations. The chemical synthesis was based on the coupling reaction of 6-hydrazinylpyridine-3-carboxylic acid with a 14-amino-acid cyclic peptide. iPD-L1 was prepared for ^99mTc labeling. Radio-HPLC was used to verify radiochemical purity. The stability of the radiopeptide in human serum was evaluated by HPLC. iPD-L1 specificity was assessed by SDS-PAGE. [^99mTc]Tc-iPD-L1 cellular uptake in PD-L1-positive cancer cells (HCC827 and HCT116) and biodistribution in mice with induced tumors were also performed. One patient with advanced plantar malignant melanoma received [^99mTc]Tc-iPD-L1. The iPD-L1 ligand (AutoDock affinity: -6.7 kcal/mol), characterized by UPLC mass, FT-IR, and UV-Vis spectroscopy, was obtained with a chemical purity of 97%. The [^99mTc]Tc-iPD-L1 was prepared with a radiochemical purity of >90%. In vitro and in vivo analyses demonstrated [^99mTc]Tc-iPD-L1 stability (>90% at 24 h) in human serum, specific recognition for PD-L1, high uptake by the tumor (6.98 ± 0.89% ID/g at 1 h), and rapid hepatobiliary and kidney elimination. [^99mTc]Tc-iPD-L1 successfully detected PD-L1-positive lesions in a patient with plantar malignant melanoma. The results obtained in this study warrant further dosimetric and clinical studies to determine the sensitivity and specificity of [^99mTc]Tc-iPD-L1/SPECT for PD-L1 expression imaging.

Keywords: PD-L1; PD-L1 imaging; PD-L1 peptide inhibitor; SPECT; technetium-99m.

Grants and funding

FICDTEM-2023-152/Consejo Mexiquense de Ciencia y Tecnología (COMECyT), EDOMEX