1. Structural Determinants of A3 Adenosine Receptor Activation: Nucleoside Ligands at the Agonist/Antagonist Boundary
- Author
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Kyeong Lee, Zhan-Guo Gao, Carl R. Johnson, Thibaud Biadatti, Kenneth A. Jacobson, Wangzhong Chen, Soo-Kyung Kim, Dov Barak, and Seong Gon Kim
- Subjects
Models, Molecular ,Agonist ,Adenosine ,Agonist-antagonist ,Stereochemistry ,medicine.drug_class ,Ribose ,CHO Cells ,Ligands ,Binding, Competitive ,Article ,Radioligand Assay ,Structure-Activity Relationship ,Cricetinae ,Drug Discovery ,Purinergic P1 Receptor Agonists ,medicine ,Animals ,Humans ,Spiro Compounds ,Adenosine A3 Receptor Agonists ,Adenosine A3 Receptor Antagonists ,Chemistry ,Receptor, Adenosine A3 ,Receptors, Purinergic P1 ,Stereoisomerism ,Ligand (biochemistry) ,Rats ,Purinergic P1 Receptor Antagonists ,Biochemistry ,Guanosine 5'-O-(3-Thiotriphosphate) ,Mutation ,Epoxy Compounds ,Molecular Medicine ,Nucleoside ,Adenosine A2B receptor ,medicine.drug - Abstract
Mutagenesis of the human A(3) adenosine receptor (AR) suggested that certain amino acid residues contributed differently to ligand binding and activation processes. Here we demonstrated that various adenosine modifications, including adenine substitution and ribose ring constraints, also contributed differentially to these processes. The ligand effects on cyclic AMP production in intact CHO cells expressing the A(3)AR and in receptor binding were compared. Notably, the simple 2-fluoro group alone or 2-chloro in combination with N(6)-substitution dramatically diminished the efficacy of adenosine derivatives, even converting agonist into antagonist. Other affinity-increasing substitutions, including N(6)-(3-iodobenzyl) 4 and the (Northern)-methanocarba 15, also reduced efficacy, except in combination with a flexible 5′-uronamide. 2-Cl-N(6)-(3-iodobenzyl) derivatives, both in the (N)-methanocarba (i.e., of the Northern conformation) and riboside series 18 and 5, respectively, were potent antagonists with little residual agonism. Ring-constrained 2′,3′-epoxide derivatives in both riboside and (N)-methanocarba series 13 and 21, respectively, and a cyclized (spiral) 4′,5′-uronamide derivative 14 were synthesized and found to be human A(3)AR antagonists. 14 bound potently at both human (26 nM) and rat (49 nM) A(3)ARs. A rhodopsin-based A(3)AR model, containing all domains except the C-terminal region, indicated separate structural requirements for receptor binding and activation for these adenosine analogues. Ligand docking, taking into account binding of selected derivatives at mutant A(3)ARs, featured interactions of TM3 (His95) with the adenine moiety and TMs 6 and 7 with the ribose 5′-region. The 5′-OH group of antagonist N(6)-(3-iodobenzyl)-2-chloroadenosine 5 formed a H-bond with N274 but not with S271. The 5′-substituent of nucleoside antagonists moved toward TM7 and away from TM6. The conserved Trp243 (6.48) side chain, involved in recognition of the classical (nonnucleoside) A(3)AR antagonists but not adenosine-derived ligands, displayed a characteristic movement exclusively upon docking of agonists. Thus, A(3)AR activation appeared to require flexibility at the 5′- and 3′-positions, which was diminished in (N)-methanocarba, spiro, and epoxide analogues, and was characteristic of ribose interactions at TM6 and TM7.
- Published
- 2002