TY - JOUR
T1 - Rational development of a high-affinity secretin receptor antagonist
AU - Dong, Maoqing
AU - Harikumar, Kaleeckal G.
AU - Raval, Sweta R.
AU - Milburn, Juliana E.
AU - Clark, Carolyn
AU - Alcala-Torano, Rafael
AU - Mobarec, Juan C.
AU - Reynolds, Christopher A.
AU - Ghirlanda, Giovanna
AU - Christopoulos, Arthur
AU - Wootten, Denise
AU - Sexton, Patrick M.
AU - Miller, Laurence J.
PY - 2020/7
Y1 - 2020/7
N2 - The secretin receptor is a prototypic class B GPCR with substantial and broad pharmacologic importance. The aim of this project was to develop a high affinity selective antagonist as a new and important pharmacologic tool and to aid stabilization of this receptor in an inactive conformation for ultimate structural characterization. Amino-terminal truncation of the natural 27-residue ligand reduced biological activity, but also markedly reduced binding affinity. This was rationally and experimentally overcome with lactam stabilization of helical structure and with replacement of residues with natural and unnatural amino acids. A key new step in this effort was the replacement of peptide residue Leu22 with L-cyclohexylalanine (Cha) to enhance potential hydrophobic interactions with receptor residues Leu31, Val34, and Phe92 that were predicted from molecular modeling. Alanine-replacement mutagenesis of these residues markedly affected ligand binding and biological activity. The optimal antagonist ligand, (Y10,c[E16,K20],I17,Cha22,R25)sec(6–27), exhibited high binding affinity (4 nM), similar to natural secretin, and exhibited no demonstrable biological activity to stimulate cAMP accumulation, intracellular calcium mobilization, or β-arrestin-2 translocation. It acts as an orthosteric competitive antagonist, predicted to bind within the peptide-binding groove in the receptor extracellular domain. The analogous peptide that was one residue longer, retaining Thr5, exhibited partial agonist activity, while further truncation of even a single residue (Phe6) reduced binding affinity. This sec(6–27)-based peptide will be an important new tool for pharmacological and structural studies.
AB - The secretin receptor is a prototypic class B GPCR with substantial and broad pharmacologic importance. The aim of this project was to develop a high affinity selective antagonist as a new and important pharmacologic tool and to aid stabilization of this receptor in an inactive conformation for ultimate structural characterization. Amino-terminal truncation of the natural 27-residue ligand reduced biological activity, but also markedly reduced binding affinity. This was rationally and experimentally overcome with lactam stabilization of helical structure and with replacement of residues with natural and unnatural amino acids. A key new step in this effort was the replacement of peptide residue Leu22 with L-cyclohexylalanine (Cha) to enhance potential hydrophobic interactions with receptor residues Leu31, Val34, and Phe92 that were predicted from molecular modeling. Alanine-replacement mutagenesis of these residues markedly affected ligand binding and biological activity. The optimal antagonist ligand, (Y10,c[E16,K20],I17,Cha22,R25)sec(6–27), exhibited high binding affinity (4 nM), similar to natural secretin, and exhibited no demonstrable biological activity to stimulate cAMP accumulation, intracellular calcium mobilization, or β-arrestin-2 translocation. It acts as an orthosteric competitive antagonist, predicted to bind within the peptide-binding groove in the receptor extracellular domain. The analogous peptide that was one residue longer, retaining Thr5, exhibited partial agonist activity, while further truncation of even a single residue (Phe6) reduced binding affinity. This sec(6–27)-based peptide will be an important new tool for pharmacological and structural studies.
KW - Antagonist
KW - G protein-coupled receptor
KW - Secretin
KW - Secretin receptor
UR - http://www.scopus.com/inward/record.url?scp=85082848495&partnerID=8YFLogxK
U2 - 10.1016/j.bcp.2020.113929
DO - 10.1016/j.bcp.2020.113929
M3 - Article
C2 - 32217097
AN - SCOPUS:85082848495
SN - 0006-2952
VL - 177
JO - Biochemical Pharmacology
JF - Biochemical Pharmacology
M1 - 113929
ER -