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Double Strain‐Promoted Macrocyclization for the Rapid Selection of Cell‐Active Stapled Peptides
Authors:Dr. Maxim Rossmann  Dr. Ban Xiong Tan  Dr. Peterson de Andrade  Dr. Yaw Sing Tan  Dr. Chandra Verma  Dr. Grahame J. McKenzie  Prof. Ashok R. Venkitaraman  Dr. Marko Hyvönen  Prof. David R. Spring
Affiliation:1. Department of Biochemistry, University of Cambridge, 80 Tennis Court Rd, Cambridge CB2 1GA (UK);2. p53Lab, A*STAR, 8A Biomedical Grove, #06‐04/05 Neuros/Immunos, Singapore 138648 (Singapore);3. Department of Chemistry, University of Cambridge, Lensfield Rd, Cambridge CB2 1EW (UK);4. Bioinformatics Institute, A*STAR, 30 Biopolis St, #07‐01 Matrix, Singapore 138671 (Singapore);5. Department of Biological Sciences, National University of Singapore, 14 Science Drive 4, Singapore 117543;6. School of Biological Sciences, Nanyang Technological University, 50 Nanyang Drive, Singapore 637551;7. Hutchison/MRC Research Centre, Hills Rd, Cambridge CB2 0XZ (UK)
Abstract:Peptide stapling is a method for designing macrocyclic alpha‐helical inhibitors of protein–protein interactions. However, obtaining a cell‐active inhibitor can require significant optimization. We report a novel stapling technique based on a double strain‐promoted azide–alkyne reaction, and exploit its biocompatibility to accelerate the discovery of cell‐active stapled peptides. As a proof of concept, MDM2‐binding peptides were stapled in parallel, directly in cell culture medium in 96‐well plates, and simultaneously evaluated in a p53 reporter assay. This in situ stapling/screening process gave an optimal candidate that showed improved proteolytic stability and nanomolar binding to MDM2 in subsequent biophysical assays. α‐Helicity was confirmed by a crystal structure of the MDM2‐peptide complex. This work introduces in situ stapling as a versatile biocompatible technique with many other potential high‐throughput biological applications.
Keywords:bioorthogonal chemistry  click chemistry  macrocycles  peptides  peptide stapling
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