In Vitro Mutational and Bioinformatics Analysis of the M71 Odorant Receptor and Its Superfamily

We performed an extensive mutational analysis of the canonical mouse odorant receptor (OR) M71 to determine the properties of ORs that inhibit plasma membrane trafficking in heterologous expression systems. We employed the use of the M71::GFP fusion protein to directly assess plasma membrane localiz...

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Autores principales: Bubnell, Jaclyn, Jamet, Sophie, Tomoiaga, Delia, D’Hulst, Charlotte, Krampis, Konstantinos, Feinstein, Paul
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2015
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4626375/
https://www.ncbi.nlm.nih.gov/pubmed/26513476
http://dx.doi.org/10.1371/journal.pone.0141712
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author Bubnell, Jaclyn
Jamet, Sophie
Tomoiaga, Delia
D’Hulst, Charlotte
Krampis, Konstantinos
Feinstein, Paul
author_facet Bubnell, Jaclyn
Jamet, Sophie
Tomoiaga, Delia
D’Hulst, Charlotte
Krampis, Konstantinos
Feinstein, Paul
author_sort Bubnell, Jaclyn
collection PubMed
description We performed an extensive mutational analysis of the canonical mouse odorant receptor (OR) M71 to determine the properties of ORs that inhibit plasma membrane trafficking in heterologous expression systems. We employed the use of the M71::GFP fusion protein to directly assess plasma membrane localization and functionality of M71 in heterologous cells in vitro or in olfactory sensory neurons (OSNs) in vivo. OSN expression of M71::GFP show only small differences in activity compared to untagged M71. However, M71::GFP could not traffic to the plasma membrane even in the presence of proposed accessory proteins RTP1S or mβ2AR. To ask if ORs contain an internal “kill sequence”, we mutated ~15 of the most highly conserved OR specific amino acids not found amongst the trafficking non-OR GPCR superfamily; none of these mutants rescued trafficking. Addition of various amino terminal signal sequences or different glycosylation motifs all failed to produce trafficking. The addition of the amino and carboxy terminal domains of mβ2AR or the mutation Y289A in the highly conserved GPCR motif NPxxY does not rescue plasma membrane trafficking. The failure of targeted mutagenesis on rescuing plasma membrane localization in heterologous cells suggests that OR trafficking deficits may not be attributable to conserved collinear motifs, but rather the overall amino acid composition of the OR family. Thus, we performed an in silico analysis comparing the OR and other amine receptor superfamilies. We find that ORs contain fewer charged residues and more hydrophobic residues distributed throughout the protein and a conserved overall amino acid composition. From our analysis, we surmise that it may be difficult to traffic ORs at high levels to the cell surface in vitro, without making significant amino acid modifications. Finally, we observed specific increases in methionine and histidine residues as well as a marked decrease in tryptophan residues, suggesting that these changes provide ORs with special characteristics needed for them to function in olfactory neurons.
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spelling pubmed-46263752015-11-06 In Vitro Mutational and Bioinformatics Analysis of the M71 Odorant Receptor and Its Superfamily Bubnell, Jaclyn Jamet, Sophie Tomoiaga, Delia D’Hulst, Charlotte Krampis, Konstantinos Feinstein, Paul PLoS One Research Article We performed an extensive mutational analysis of the canonical mouse odorant receptor (OR) M71 to determine the properties of ORs that inhibit plasma membrane trafficking in heterologous expression systems. We employed the use of the M71::GFP fusion protein to directly assess plasma membrane localization and functionality of M71 in heterologous cells in vitro or in olfactory sensory neurons (OSNs) in vivo. OSN expression of M71::GFP show only small differences in activity compared to untagged M71. However, M71::GFP could not traffic to the plasma membrane even in the presence of proposed accessory proteins RTP1S or mβ2AR. To ask if ORs contain an internal “kill sequence”, we mutated ~15 of the most highly conserved OR specific amino acids not found amongst the trafficking non-OR GPCR superfamily; none of these mutants rescued trafficking. Addition of various amino terminal signal sequences or different glycosylation motifs all failed to produce trafficking. The addition of the amino and carboxy terminal domains of mβ2AR or the mutation Y289A in the highly conserved GPCR motif NPxxY does not rescue plasma membrane trafficking. The failure of targeted mutagenesis on rescuing plasma membrane localization in heterologous cells suggests that OR trafficking deficits may not be attributable to conserved collinear motifs, but rather the overall amino acid composition of the OR family. Thus, we performed an in silico analysis comparing the OR and other amine receptor superfamilies. We find that ORs contain fewer charged residues and more hydrophobic residues distributed throughout the protein and a conserved overall amino acid composition. From our analysis, we surmise that it may be difficult to traffic ORs at high levels to the cell surface in vitro, without making significant amino acid modifications. Finally, we observed specific increases in methionine and histidine residues as well as a marked decrease in tryptophan residues, suggesting that these changes provide ORs with special characteristics needed for them to function in olfactory neurons. Public Library of Science 2015-10-29 /pmc/articles/PMC4626375/ /pubmed/26513476 http://dx.doi.org/10.1371/journal.pone.0141712 Text en © 2015 Bubnell et al http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Bubnell, Jaclyn
Jamet, Sophie
Tomoiaga, Delia
D’Hulst, Charlotte
Krampis, Konstantinos
Feinstein, Paul
In Vitro Mutational and Bioinformatics Analysis of the M71 Odorant Receptor and Its Superfamily
title In Vitro Mutational and Bioinformatics Analysis of the M71 Odorant Receptor and Its Superfamily
title_full In Vitro Mutational and Bioinformatics Analysis of the M71 Odorant Receptor and Its Superfamily
title_fullStr In Vitro Mutational and Bioinformatics Analysis of the M71 Odorant Receptor and Its Superfamily
title_full_unstemmed In Vitro Mutational and Bioinformatics Analysis of the M71 Odorant Receptor and Its Superfamily
title_short In Vitro Mutational and Bioinformatics Analysis of the M71 Odorant Receptor and Its Superfamily
title_sort in vitro mutational and bioinformatics analysis of the m71 odorant receptor and its superfamily
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4626375/
https://www.ncbi.nlm.nih.gov/pubmed/26513476
http://dx.doi.org/10.1371/journal.pone.0141712
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