Identification of an Arg-Leu-Arg tripeptide that contributes to the binding interface between the cytokine MIF and the chemokine receptor CXCR4

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作者
Michael Lacy
Christos Kontos
Markus Brandhofer
Kathleen Hille
Sabine Gröning
Dzmitry Sinitski
Priscila Bourilhon
Eric Rosenberg
Christine Krammer
Tharshika Thavayogarajah
Georgios Pantouris
Maria Bakou
Christian Weber
Elias Lolis
Jürgen Bernhagen
Aphrodite Kapurniotu
机构
[1] Institute for Stroke and Dementia Research,Department of Vascular Biology
[2] Klinikum der Universität München,Division of Peptide Biochemistry
[3] Ludwig-Maximilians-University of Munich,Department of Anaesthesiology
[4] Technische Universität München,Department of Pharmacology
[5] RWTH Aachen University Hospital,Institute for Cardiovascular Prevention
[6] Yale University School of Medicine,Cardiovascular Research Institute Maastricht
[7] Klinikum der Universität München,undefined
[8] Ludwig-Maximilians-University of Munich,undefined
[9] Munich Heart Alliance,undefined
[10] Maastricht University,undefined
[11] Munich Cluster for Systems Neurology,undefined
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MIF is a chemokine-like cytokine that plays a role in the pathogenesis of inflammatory and cardiovascular disorders. It binds to the chemokine-receptors CXCR2/CXCR4 to trigger atherogenic leukocyte migration albeit lacking canonical chemokine structures. We recently characterized an N-like-loop and the Pro-2-residue of MIF as critical molecular determinants of the CXCR4/MIF binding-site and identified allosteric agonism as a mechanism that distinguishes CXCR4-binding to MIF from that to the cognate ligand CXCL12. By using peptide spot-array technology, site-directed mutagenesis, structure-activity-relationships, and molecular docking, we identified the Arg-Leu-Arg (RLR) sequence-region 87–89 that – in three-dimensional space – ‘extends’ the N-like-loop to control site-1-binding to CXCR4. Contrary to wildtype MIF, mutant R87A-L88A-R89A-MIF fails to bind to the N-terminal of CXCR4 and the contribution of RLR to the MIF/CXCR4-interaction is underpinned by an ablation of MIF/CXCR4-specific signaling and reduction in CXCR4-dependent chemotactic leukocyte migration of the RLR-mutant of MIF. Alanine-scanning, functional competition by RLR-containing peptides, and molecular docking indicate that the RLR residues directly participate in contacts between MIF and CXCR4 and highlight the importance of charge-interactions at this interface. Identification of the RLR region adds important structural information to the MIF/CXCR4 binding-site that distinguishes this interface from CXCR4/CXCL12 and will help to design MIF-specific drug-targeting approaches.
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