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« Previous AbstractOptimization of Headspace Solid-Phase Micro-Extraction Conditions (HS-SPME) and Identification of Major Volatile Aroma-Active Compounds in Chinese Chive (Allium tuberosum Rottler)    Next AbstractSynthesis and biological evaluation of the geometric farnesylated analogues of the a-factor mating peptide of Saccharomyces cerevisiae »

J Pept Res


Title:"Structure, biological activity and membrane partitioning of analogs of the isoprenylated a-factor mating peptide of Saccharomyces cerevisiae"
Author(s):Xie H; Becker JM; Gibbs RA; Naider F;
Address:"Department of Chemistry, The College of Staten Island and The Graduate School of The City University of New York, Staten Island, USA"
Journal Title:J Pept Res
Year:2000
Volume:55
Issue:5
Page Number:372 - 383
DOI: 10.1034/j.1399-3011.2000.00705.x
ISSN/ISBN:1397-002X (Print) 1397-002X (Linking)
Abstract:"Previous biochemical investigations on the Saccharomyces cerevisiae a-factor indicated that this lipopeptide pheromone [YIIKGVFWDPAC(farnesyl)OMe] might adopt a type II beta-turn at positions 4 and 5 of the peptide sequence. To test this hypothesis, we synthesized five analogs of a-factor, in which residues at positions 4 and 5 were replaced with: L-Pro4(I); D-Pro4(II); L-Pro4-D-Ala5(III); D-Pro4-L-Ala5(IV); or Nle4(V). Analogs were purified to > 99% homogeneity as evidenced by HPLC and TLC and were characterized by mass spectrometry and amino acid analysis. Using a growth arrest assay the conformationally restricted a-factor analogs I and III were found to be almost 50-fold more active than the diastereometric homologs II and IV and were equally active to wild-type a-factor. Replacement of Lys4 with the isosteric Nle4 almost abolished the activity of the pheromone. Thus, the incorporation of residues that promote a type II beta-turn compensated for the loss of the favorable contribution of the Lys4 side chain to pheromone activity. CD spectra on these peptides suggested that they were essentially disordered in both TFE/H2O and in the presence of DMPC vesicles. There was no correlation between CD peak shape and biological activity. Using fluorescence spectroscopy we measured the interaction of lipid vesicles with these position 4 and 5 analogs as well as with three a-factor analogs with a modified farnesyl group. The results indicated that modifications of both the peptide sequence and the lipid moiety affect partitioning into lipid, and that no correlation existed between the propensity of a pheromone to partition into the lipid and its biological activity"
Keywords:"Cell Division Cell Membrane/*chemistry Chromatography, High Pressure Liquid Circular Dichroism Dose-Response Relationship, Drug Mating Factor Models, Chemical Peptide Biosynthesis Peptides/*chemistry Pheromones/*chemistry Protein Binding *Protein Prenylat;"
Notes:"MedlineXie, H Becker, J M Gibbs, R A Naider, F eng CA-78819/CA/NCI NIH HHS/ GM-22086/GM/NIGMS NIH HHS/ GM-22087/GM/NIGMS NIH HHS/ Research Support, U.S. Gov't, P.H.S. Denmark 2000/06/23 J Pept Res. 2000 May; 55(5):372-83. doi: 10.1034/j.1399-3011.2000.00705.x"

 
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