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« Previous AbstractCharacterization of Key Odorants Causing a Fusty/Musty Off-Flavor in Native Cold-Pressed Rapeseed Oil by Means of the Sensomics Approach    Next AbstractA Novel Screening Approach for Optimal and Functional Fusion of T4 Lysozyme in GPCRs »

Protein Eng Des Sel


Title:Functional fusions of T4 lysozyme in the third intracellular loop of a G protein-coupled receptor identified by a random screening approach in yeast
Author(s):Mathew E; Ding FX; Naider F; Dumont ME;
Address:"Department of Biochemistry and Biophysics, University of Rochester School of Medicine and Dentistry, Rochester, NY 14642, USA"
Journal Title:Protein Eng Des Sel
Year:2013
Volume:20121016
Issue:1
Page Number:59 - 71
DOI: 10.1093/protein/gzs070
ISSN/ISBN:1741-0134 (Electronic) 1741-0126 (Print) 1741-0126 (Linking)
Abstract:"The insertion of a stable soluble protein into loops of transmembrane proteins has proved to be a successful approach for enhancing their stabilities and crystallization, and may also be useful in contexts where the inserted proteins can modulate or report on the activities of membrane proteins. While the use of T4 lysozyme to replace portions of the third intracellular loops of G protein-coupled receptors (GPCRs) has allowed determination of the structures of members of this important class of receptors, the creation of such fusion proteins generally leads to loss of signaling function of the resulting fusion protein, since the third intracellular loops of GPCRs play critical roles in their interactions with G proteins. We describe here a random screening approach allowing insertion of T4 lysozyme into diverse positions in the third loop of the yeast alpha-pheromone receptor, a GPCR encoded by the yeast STE2 gene. Insertions were accompanied by varying extents of deletion or duplication of the loop. A set of phenotypic screens allow detection of potentially rare variant receptors that are expressed, bind to agonist and are capable of signal transduction via activation of the cognate G protein. A large fraction of screened full-length receptor variants containing at least partial duplications of the loop on either side of the inserted T4 lysozyme retain the ability to activate the downstream signaling pathway in response to binding of ligand. However, we were unable to identify any receptors with truncated C-termini that retain significant signaling function in the presence of inserted T4 lysozyme. Our results establish the feasibility of creating functional receptors containing insertions of T4 lysozyme in their third intracellular loops"
Keywords:"Amino Acid Sequence Bacteriophage T4/*enzymology/genetics Base Sequence Gene Library Intracellular Space/*metabolism Ligands Molecular Sequence Data Muramidase/*genetics Protein Engineering/*methods Receptors, G-Protein-Coupled/*chemistry/genetics/*metabo;"
Notes:"MedlineMathew, Elizabeth Ding, Fa-Xiang Naider, Fred Dumont, Mark E eng GM084083/GM/NIGMS NIH HHS/ GM22086/GM/NIGMS NIH HHS/ Research Support, N.I.H., Extramural England 2012/10/19 Protein Eng Des Sel. 2013 Jan; 26(1):59-71. doi: 10.1093/protein/gzs070. Epub 2012 Oct 16"

 
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