The present study describes a small library of peptides derived from a potent and selective CXCR4 antagonist (3), 3 ), wherein the native disulfide bond is replaced using a side-chain to tail macrolactamization technique to vary ring size and amino acid composition. The peptides were preliminary assessed for their ability to interfere with the interaction between the receptor and anti-CXCR4 PE-conjugated antibody clone 12G5. Two promising candidates (13 13 and 17 ) were identified and further evaluated in a125I-CXCL12 125 I-CXCL12 competition binding assay, exhibiting IC50 50 in the low-nanomolar range. Furthermore, both candidates displayed high selectivity towards CXCR4 with respect to the cognate receptor CXCR7, ability to block CXCL12-dependent cancer cell migration, and receptor internalization, albeit at a higher concentration compared to 3 . Molecular modeling studies on 13 and 17 produced a theoretical model that may serve as a guide for future modifications, aiding in the development of analogs with improved affinity. Finally, the study provides valuable insights into developing therapeutic agents targeting CXCR4-mediated processes, demonstrating the adaptability of our lead peptide 3 to alternative cyclization approaches and offering prospects for comprehensive investigations into the receptor region's interaction with its C-terminal region.

Disulfide bond replacement with non-reducible side chain to tail macrolactamization for the development of potent and selective CXCR4 peptide antagonists endowed with flanking binding sites

Messere, Anna;D'Aniello, Antonia;Del Bene, Alessandra;Roggia, Michele;Cutolo, Roberto;Campagna, Erica;Russo, Rosita;Chambery, Angela;Benedetti, Rosaria;Altucci, Lucia;Cosconati, Sandro;Di Maro, Salvatore
2024

Abstract

The present study describes a small library of peptides derived from a potent and selective CXCR4 antagonist (3), 3 ), wherein the native disulfide bond is replaced using a side-chain to tail macrolactamization technique to vary ring size and amino acid composition. The peptides were preliminary assessed for their ability to interfere with the interaction between the receptor and anti-CXCR4 PE-conjugated antibody clone 12G5. Two promising candidates (13 13 and 17 ) were identified and further evaluated in a125I-CXCL12 125 I-CXCL12 competition binding assay, exhibiting IC50 50 in the low-nanomolar range. Furthermore, both candidates displayed high selectivity towards CXCR4 with respect to the cognate receptor CXCR7, ability to block CXCL12-dependent cancer cell migration, and receptor internalization, albeit at a higher concentration compared to 3 . Molecular modeling studies on 13 and 17 produced a theoretical model that may serve as a guide for future modifications, aiding in the development of analogs with improved affinity. Finally, the study provides valuable insights into developing therapeutic agents targeting CXCR4-mediated processes, demonstrating the adaptability of our lead peptide 3 to alternative cyclization approaches and offering prospects for comprehensive investigations into the receptor region's interaction with its C-terminal region.
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/11591/534148
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