Concentration of 200 mM) or as a mixture (L-arginine, L-lysine and L-methionine; each at 200 mM). All amino acids and bath solution chemicals were purchased from Sigma (Deisenhofen, Germany). Peptides consisting of selected combinations of L-arginine, L-methionine, L-lysine (group I peptides) and L-arginine, L-methionine, Fruquintinib glycine (group II peptides) were purchased from GenScript (Piscataway, NJ, USA; L-arginyl-L-methionine, L-methionyl-L-arginine, L-arginyl-L-methionyl-L-arginine, L-methionyl-L-arginyl-L-methionine, L-arginyl-L-lysine, L-lysyl-L-arginine, L-arginyl-L-lysyl-L-arginine, Llysyl-L-arginyl-L-lysine, glycyl-L-arginine, L-arginyl-glycine) or Sigma (L-methionyl-glycine, glycyl-glycine, glycyl-glycyl-glycine). Tissue slices (see above) were transferred to a recording chamber, and 200 ml of bath solution containing 50 mM Fluo-4/AM (Molecular Probes, Leiden, The Netherlands) was added. Fluo4/AM was dissolved in DMSO (Sigma) and Pluronic F-127 (Molecular Probes). The final concentrations of DMSO and Pluronic F-127 did not exceed 0.5 and 0.1 , respectively. Cells of the OE of larval Xenopus laevis express multidrug resistance transporters with a wide substrate spectrum, including Ca2+indicator dyes [29,30]. To avoid transporter-mediated destaining of the slices, 50 mM MK571 (Alexis Biochemicals, Grunberg, ?Germany), an inhibitor of multidrug transporters, was added to the incubation solution. The preparations were incubated on a shaker at room temperature for 35 minutes. During the experiment, the recording chamber was constantly perfused with bath solution applied by gravity feed from a storage syringe through a funnel drug applicator. The flow rate was 350 ml min21. The tip of the applicator was placed directly above the OE. Before starting the experiments the slices were rinsed with bath solution for at least five minutes. After the first ten frames of each recording, amino acids and peptides were applied into the funnel in random order without stopping the bath solution flow. Bath solution was removed from the recording chamber through a syringe needle placed close to the OE. All experiments were conducted at room temperature. The reproducibility of peptide responses was verified by MedChemExpress UKI 1 regularly repeating the application at least twice. To ensure sustained cell viability amino acids as positive control were regularly applied during and at the end of all experiments. The minimum interstimulus interval was at least two minutes in all of the experiments.Ca2+ imaging and data evaluationChanges of intracellular calcium concentrations of individual ORNs were monitored using a laser-scanning confocal microscopeFigure 1. Amino acid- and peptide-induced changes in calcium-dependent fluorescence of individual ORNs in slices of the olfactory epithelium. (A) Slice preparation 1527786 of the OE of larval Xenopus laevis stained with Fluo-4 AM. The colored ovals (#1?8) indicate the eight ORNs that were responsive to the mixture of amino acids. (B) Time courses of [Ca2+]i transients of the eight ORNs marked in A, elicited by application of amino acids (L-arginine, L-methionine and L-lysine as a mixture or singularly; each at a concentration of 200 mM) and peptides (consisting of L-arginine, Lmethionine and L-lysine; 200 mM and 1 mM). Discernible peptide induced [Ca2+]i transients are marked by an asterisk. To check for ORN viability, the mixture of amino acids was applied at the end of the experiment. (C) Examples of peptide induced calcium transients o.Concentration of 200 mM) or as a mixture (L-arginine, L-lysine and L-methionine; each at 200 mM). All amino acids and bath solution chemicals were purchased from Sigma (Deisenhofen, Germany). Peptides consisting of selected combinations of L-arginine, L-methionine, L-lysine (group I peptides) and L-arginine, L-methionine, glycine (group II peptides) were purchased from GenScript (Piscataway, NJ, USA; L-arginyl-L-methionine, L-methionyl-L-arginine, L-arginyl-L-methionyl-L-arginine, L-methionyl-L-arginyl-L-methionine, L-arginyl-L-lysine, L-lysyl-L-arginine, L-arginyl-L-lysyl-L-arginine, Llysyl-L-arginyl-L-lysine, glycyl-L-arginine, L-arginyl-glycine) or Sigma (L-methionyl-glycine, glycyl-glycine, glycyl-glycyl-glycine). Tissue slices (see above) were transferred to a recording chamber, and 200 ml of bath solution containing 50 mM Fluo-4/AM (Molecular Probes, Leiden, The Netherlands) was added. Fluo4/AM was dissolved in DMSO (Sigma) and Pluronic F-127 (Molecular Probes). The final concentrations of DMSO and Pluronic F-127 did not exceed 0.5 and 0.1 , respectively. Cells of the OE of larval Xenopus laevis express multidrug resistance transporters with a wide substrate spectrum, including Ca2+indicator dyes [29,30]. To avoid transporter-mediated destaining of the slices, 50 mM MK571 (Alexis Biochemicals, Grunberg, ?Germany), an inhibitor of multidrug transporters, was added to the incubation solution. The preparations were incubated on a shaker at room temperature for 35 minutes. During the experiment, the recording chamber was constantly perfused with bath solution applied by gravity feed from a storage syringe through a funnel drug applicator. The flow rate was 350 ml min21. The tip of the applicator was placed directly above the OE. Before starting the experiments the slices were rinsed with bath solution for at least five minutes. After the first ten frames of each recording, amino acids and peptides were applied into the funnel in random order without stopping the bath solution flow. Bath solution was removed from the recording chamber through a syringe needle placed close to the OE. All experiments were conducted at room temperature. The reproducibility of peptide responses was verified by regularly repeating the application at least twice. To ensure sustained cell viability amino acids as positive control were regularly applied during and at the end of all experiments. The minimum interstimulus interval was at least two minutes in all of the experiments.Ca2+ imaging and data evaluationChanges of intracellular calcium concentrations of individual ORNs were monitored using a laser-scanning confocal microscopeFigure 1. Amino acid- and peptide-induced changes in calcium-dependent fluorescence of individual ORNs in slices of the olfactory epithelium. (A) Slice preparation 1527786 of the OE of larval Xenopus laevis stained with Fluo-4 AM. The colored ovals (#1?8) indicate the eight ORNs that were responsive to the mixture of amino acids. (B) Time courses of [Ca2+]i transients of the eight ORNs marked in A, elicited by application of amino acids (L-arginine, L-methionine and L-lysine as a mixture or singularly; each at a concentration of 200 mM) and peptides (consisting of L-arginine, Lmethionine and L-lysine; 200 mM and 1 mM). Discernible peptide induced [Ca2+]i transients are marked by an asterisk. To check for ORN viability, the mixture of amino acids was applied at the end of the experiment. (C) Examples of peptide induced calcium transients o.