A different molecular interaction of bradykinin and the synthetic agonist FR190997 with the human B2 receptor: evidence from mutational analysis

Francesca Bellucci; Stefania Meini; Paola Cucchi; Claudio Catalani; Wolfgang Reichert; Sabrina Zappitelli; Luigi Rotondaro; Laura Quartara; Alessandro Giolitti; Carlo Alberto Maggi

doi:10.1038/sj.bjp.0705454

A different molecular interaction of bradykinin and the synthetic agonist FR190997 with the human B2 receptor: evidence from mutational analysis

Br J Pharmacol. 2003 Oct;140(3):500-6. doi: 10.1038/sj.bjp.0705454. Epub 2003 Aug 26.

Authors

Francesca Bellucci¹, Stefania Meini, Paola Cucchi, Claudio Catalani, Wolfgang Reichert, Sabrina Zappitelli, Luigi Rotondaro, Laura Quartara, Alessandro Giolitti, Carlo Alberto Maggi

Affiliation

¹ Department of Pharmacology, Menarini Ricerche S.p.A., via Rismondo 12A, Florence 50131, Italy.

Abstract

Binding affinity at the [3H]-BK binding site and activity as inositol phosphate (IP) production by the peptide bradykinin (BK) and the nonpeptide FR190997 were studied at wild-type or point-mutated human B2 receptors (hB2R) expressed in CHO cells. The effect of the following mutations were analyzed: E47A (TM1), W86A and T89A (TM2), I110A, L114A and S117A (TM3), T158A, M165T and L166F (TM4), T197A and S211A (TM5), F252A, W256A and F259A (TM6), S291A, F292A, Y295A and Y295F (TM7), and the double mutation W256A/Y295F. As the wild-type receptor-binding affinity of FR190997 was 40-fold lower than BK, whereas their agonist potency was comparable, both agonists produced similar maximal effects (Emax). Mutations were evaluated as affecting the affinity and/or efficacy of FR190997 compared with BK. Two mutations were found to impair the agonist affinity of both agonists drastically: W86A and F259A. BK agonist affinity (pEC50) was reduced by 1400- and 150-fold, and that of FR190997 was reduced by 400- and 25-fold, at the W86A and F259A mutant B2 receptors, respectively. Contrary to BK, the affinity of FR190997 was selectively decreased at I110A, Y295A, and Y295F mutants (>103-fold), and a different efficacy was measured at the Y295 mutants, FR190997 being devoid of the capability to trigger IP production at Y295A mutant. L114A, F252A, and W256A selectively impaired the efficacy of FR190997, whereas its binding affinity was not affected. As a consequence, FR190997 behaved as a high-affinity antagonist in blocking the IP production induced by BK. The lack of capability of FR190997 to activate or to bind the double mutant W256A/Y295F suggests that these residues are part of the same binding site, which is also important for receptor activation by the nonpeptide ligand. Overall, by means of mutational analysis, we indicate an hB2R recognition site for the nonpeptide agonist FR190997 (between TM3, 6, and 7), different from that of BK, and show that in the same binding crevice some mutations (L114, W256, and F252) are selectively responsible for the agonist properties of only FR190997.

Publication types

Comparative Study

MeSH terms

Animals
Bradykinin / metabolism*
CHO Cells
Cricetinae
DNA Mutational Analysis / methods
Dose-Response Relationship, Drug
Humans
Mutation
Protein Binding / physiology
Quinolines / metabolism*
Receptor, Bradykinin B2 / agonists
Receptor, Bradykinin B2 / genetics*
Receptor, Bradykinin B2 / metabolism*

Substances

FR 190997
Quinolines
Receptor, Bradykinin B2
Bradykinin