Corinna Morys-Wortmann scite author profile

Glucagon-like peptide-1 is a gastrointestinal hormone that strongly stimulates insulin release via specific receptors on the pancreatic p-cell. To characterize the side-chain groups required for interaction of glucagon-like peptide-1 with its receptor, we performed binding studies with alanine-substituted glucagon-like peptide-1 analogues on RINmSF insulinoma cells. The binding affinity and biological activity of glucagon-like peptide-1 have been found to be sensitive to alanine exchanges in the N-terminal positions 1, 4, 6 and the C-terminal positions 22 and 23. Alanine substitutions at positions 5, 8, 10-12, 14, 16-21 and 25-30 do not change receptor affinity. These findings could be exploited to design glucagon-like peptide-1 agonists and probably antagonists for further physiological studies.Glucagon-like peptide-1 is a 30-residue gastrointestinal hormone released from the enteroglucagon cells (L-cells) in the small intestine [l -31. The post-translational processing of proglucagon in the small intestine leads to the generation of glucagon-like peptide-1, corresponding to positions 78 -108 of the human proglucagon precursor [3, 41. In v i m , glucagon-like peptide-1 increases insulin secretion from the isolated rat [S] and pig pancreas [2, 61, and from isolated rat islets [7]. In man, glucagon-like peptide-1 is released into the circulation postprandially, and glucagon-like peptide-1 infusions stimulate insulin release [ 81. Therefore, glucagon-like peptide-1 plays an important role in the postprandial regulation of insulin secretion. Recent studies have shown that glucagon-like peptide-1 also has an anti-diabetogenic effect by reducing the isoglycaemic meal-related requirement for insulin in patients with non-insulin-dependent diabetes mellitus [9][10][11].Receptors for glucagon-like peptide-1 have been characterized in RINm5F cells [12-141, a Abbreviations. Fmoc, N-9-fluorenylmethoxycarbonyl; [HlAIglucagon-like peptide-1 , glucagon-like peptide-I , with an alanine exchange in position 1 for the naturally occurring histidine residue. All other glucagon-like peptide-1 analogues are named accordingly with the first letter giving the naturally occurring amino acid in the glucagon-like peptide-1 sequence and the number following the first letter giving the position of the exchanged amino acid.Note. This work is dedicated to Werner Creutzfeldt, Professor emeritus of Medicine, Georg-August University of Gottingen, Germany, on the occasion of his 70th birthday. the gene encoding the receptor has been localized in humans [17]. So far, little is known about the structural requirements for glucagon-like peptide-1 binding to its receptor. Binding studies with N-terminal and C-terminal glucagon-like peptide-1 fragments have shown that the C-terminal domains of the glucagon-like peptide-1 molecule are important for receptor binding. The N-terminal fragment glucagon-like peptide-1 (7 -2.5) did not show receptor binding, indicating that longer N-terminal fragments are needed for receptor recognition [ 1 31. The glucag...

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Biological activity of GLP-1-analogues with N-terminal modifications

Siegel

Gallwitz

Scharf

et al. 1999

Regulatory Peptides

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GLP-1-analogues resistant to degradation by dipeptidyl-peptidase IV in vitro

Gallwitz

Ropeter

Morys-Wortmann

et al. 2000

Regulatory Peptides

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Channel Active Mammalian Porin, Purified from Crude Membrane Fractions of Human B Lymphocytes and Bovine Skeletal Muscle, Reversibly Binds Adenosine Triphosphate (ATP)

Flörke¹,

Thinnes²,

Winkelbach³

et al. 1994

Biological Chemistry Hoppe-Seyler

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A new aspect of mammalian porin (mammalian VDAC = mammalian voltage-dependent anion channel) is presented: channel active VDAC binds adenosine triphosphate (ATP) in the absence of Ca2+. Channel active "Porin 31HL" or "Porin 31BM", enriched from crude membranes of human B lymphocytes or whole cell lysates of bovine skeletal muscle, respectively, was bound to a nine atoms spacer ATP-agarose at pH 7.4 or 5.0 and reeluted from the resin by 10 mM ATP disodium salt. Furthermore, channel active "Porin 31BM" was labelled by [32P]ATP in a 1:1 stoichiometric relation. Binding of ATP to human porin was confirmed by studying the interaction of the synthetic porin fragment Type-1/Ac-35, comprising the putative nucleotide binding site G Y G F G, with trinitrophenyl-ATP (TNT-ATP) by scanning fluorometry. Peptide/TNP-ATP complexes clearly show enhancement of fluorescence intensity and a spectral shift of the fluorescence maximum. In a control experiment, using a porin fragment lacking the putative nucleotide binding site, no change of fluorescence emission was observed. Further confirmation for ATP binding by human VDAC arose from an autoradiographic experimental approach: the porin fragment Type-1/Ac-35 could be labelled by [32P]ATP, while a second porin fragment ending immediately before the putative nucleotide binding site could not; nor could a synthetic non porin peptide.

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Relaxant effect of xenin on rat ileum is mediated by apamin-sensitive neurotensin-type receptors

Clemens

Katsoulis

Nustede

et al. 1997

American Journal of Physiology-Gastrointestinal and Liver Physi

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The action of xenin, a novel 25-residue peptide of the neurotensin (NT)/xenopsin family, was investigated in isolated rat ileal muscle strips and in dispersed longitudinal smooth muscle cells of rat small intestine in vitro. Xenin relaxes KCl-precontracted ileal strips dose dependently (1 nM-3 microM). The order of potency of the investigated peptides was as follows: xenopsin = NT = xenin > neuromedin N. Kinetensin was inactive. Tetrodotoxin, hexamethonium, tetraethylammonium, 4-aminopyridine, and NG-nitro-L-arginine did not influence the relaxant effects of xenin or NT, whereas the K+ channel blocker apamin nearly abolished their effects. Desensitization against one of the peptides or blockade of NT receptors by SR-48692 prevented the effect of xenin and NT. Structure-activity experiments revealed that the COOH-terminal part of the molecules of xenin and NT is essential for biological activity. Experiments with isolated dispersed smooth muscle cells and binding studies on intestinal smooth muscle cell membranes confirmed and extended the results obtained with muscle strips. In conclusion, xenin relaxes rat ileal smooth muscle via a muscular NT-type apamin-sensitive receptor.

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