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Heimbrook DC, Boyer ME, Garsky VM, et al. Minimal ligand analysis of gastrin releasing peptide. Receptor binding and mitogenesis. J Biol Chem. 1988;263(15):7016-9
Heimbrook, D. C., Boyer, M. E., Garsky, V. M., Balishin, N. L., Kiefer, D. M., Oliff, A., & Riemen, M. W. (1988). Minimal ligand analysis of gastrin releasing peptide. Receptor binding and mitogenesis. The Journal of biological chemistry, 263(15), 7016-9.
Heimbrook, D C, et al. "Minimal ligand analysis of gastrin releasing peptide. Receptor binding and mitogenesis." The Journal of biological chemistry vol. 263,15 (1988): 7016-9.
Heimbrook DC, Boyer ME, Garsky VM, Balishin NL, Kiefer DM, Oliff A, Riemen MW. Minimal ligand analysis of gastrin releasing peptide. Receptor binding and mitogenesis. J Biol Chem. 1988 May 25;263(15):7016-9. PMID: 2835360.
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Elsevier Science

J Biol Chem. 1988 May 25;263(15):7016-9.

Minimal ligand analysis of gastrin releasing peptide. Receptor binding and mitogenesis.

The Journal of biological chemistry

D C Heimbrook, M E Boyer, V M Garsky, N L Balishin, D M Kiefer, A Oliff, M W Riemen

Affiliations

  1. Department of Cancer Research, Merck Sharp and Dohme Research Laboratories, West Point, Pennsylvania 19486.

PMID: 2835360
Free Article

Abstract

Gastrin releasing peptide (GRP) is a peptide hormone containing 27 amino acids which is structurally analogous to the amphibian peptide bombesin. GRP serves a variety of physiological functions and has been implicated in the pathophysiology of small cell lung cancer. Previous work has demonstrated that the modified C terminus of GRP, N-acetyl-GRP-20-27, exerts full agonist activity in a variety of assay systems. However, no systematic comparison of binding of GRP fragments to its receptor and mitogenic potency has been reported. To investigate whether smaller GRP fragments could bind to the GRP receptor without stimulating mitogenesis, we performed binding inhibition and thymidine uptake assays with Swiss 3T3 fibroblasts. These studies were facilitated by the development of a novel tritiated GRP-based radioligand, [3H-Phe15] GRP-15-27, which exhibits enhanced chemical stability compared to iodinated GRP derivatives. We examined a series of C-terminal GRP fragments, from the pentapeptide to the octapeptide, with both N-acetyl and free amine moieties at the N terminus. N-Acetylated derivatives were more potent than their primary amine counterparts in both assays. Deletion of N-terminal residues from GRP-20-27 resulted in significant loss of potency in both assays: the EC50 values of N-acetyl-GRP-21-27 were 10(2)-fold higher than N-acetyl-GRP-20-27, those of N-acetyl-GRP-22-27 were 10(4)-fold higher, and N-acetyl-GRP-23-27 showed minimal activity at concentrations below 100 microM. These results suggest that 1) both His20 and Trp21 play an important role in binding of GRP to the receptor, and 2) for this series of N-terminal deletions, binding to the receptor and mitogenic activity are tightly coupled.

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