A New Peptidic Vector for Molecular Imaging of Apoptosis, Identified by Phage Display Technology

Author:

Laumonier Catherine,Segers Jérôme,Laurent Sophie1,Michel Alain2,Coppée Frédérique,Belayew Alexandra3,Elst Luce Vander1,Muller Robert N.4

Affiliation:

1. Department of General, Organic and Biomedical Chemistry, NMR and Molecular Imaging Laboratory, University of Mons-Hainaut, Mons, Belgium

2. Laboratory of Proteomic and Protein Chemistry, University of Mons-Hainaut, Mons, Belgium

3. Laboratory of Molecular Biology, University of Mons-Hainaut, Mons, Belgium

4. Department of General, Organic and Biomedical Chemistry, NMR and Molecular Imaging Laboratory, University of Mons-Hainaut 24, Avenue du Champ de Mars, B-7000 Mons, Belgium

Abstract

Phosphatidylserine (PS) exposure on the cell surface is an early marker of apoptosis. To select PS binding peptides as vectors of contrast agents to image apoptosis, a phage library has been exposed to perfused mouse livers. Phages not retained on control livers during the first perfusions were used for selections on apoptotic livers in a second series of perfusions. Four selected phages were further evaluated for binding to PS-coated enzyme-linked immunosorbent assay (ELISA) plates. They presented an apparent affinity constant (Kaapp) for PS ranging from 6.08 × 1010M to 1.62 × 1011M. These phages did not bind to phosphatidylcholine, and competition with annexin V confirmed their specific interaction with PS. The phage with the highest affinity-bound PS in ELISA with a Kaapp= (1.6 ± 0.2) × 1011M. It carried the TLVSSL peptide that was synthesized. Specific competition with annexin V and with the synthetic peptide was performed and confirms the specificity of the interaction. ( Journal of Biomolecular Screening 2006:537-545)

Publisher

Elsevier BV

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