Flow cytometry-based FRET identifies binding intensities in PPARγ1 protein-protein interactions in living cells

PPARγ is a pharmacological target in inflammatory and metabolic diseases. Upon agonistic treatment or following antagonism, binding of co-factors is altered, which consequently affects PPARγ-dependent transactivation as well as its DNA-independent properties. Therefore, establishing techniques to ch...

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Autores principales: Trümper, Verena, von Knethen, Andreas, Preuß, Annegret, Ermilov, Eugeny, Hackbarth, Steffen, Kuchler, Laura, Gunne, Sandra, Schäfer, Anne, Bornhütter, Tobias, Vereb, György, Ujlaky-Nagy, Lázló, Brüne, Bernhard, Röder, Beate, Schindler, Michael, Parnham, Michael J., Knape, Tilo
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Ivyspring International Publisher 2019
Materias:
Research Paper
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6735382/
https://www.ncbi.nlm.nih.gov/pubmed/31534496
http://dx.doi.org/10.7150/thno.29367
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author Trümper, Verena
von Knethen, Andreas
Preuß, Annegret
Ermilov, Eugeny
Hackbarth, Steffen
Kuchler, Laura
Gunne, Sandra
Schäfer, Anne
Bornhütter, Tobias
Vereb, György
Ujlaky-Nagy, Lázló
Brüne, Bernhard
Röder, Beate
Schindler, Michael
Parnham, Michael J.
Knape, Tilo
author_facet Trümper, Verena
von Knethen, Andreas
Preuß, Annegret
Ermilov, Eugeny
Hackbarth, Steffen
Kuchler, Laura
Gunne, Sandra
Schäfer, Anne
Bornhütter, Tobias
Vereb, György
Ujlaky-Nagy, Lázló
Brüne, Bernhard
Röder, Beate
Schindler, Michael
Parnham, Michael J.
Knape, Tilo
author_sort Trümper, Verena
collection PubMed
description PPARγ is a pharmacological target in inflammatory and metabolic diseases. Upon agonistic treatment or following antagonism, binding of co-factors is altered, which consequently affects PPARγ-dependent transactivation as well as its DNA-independent properties. Therefore, establishing techniques to characterize these interactions is an important issue in living cells. Methods: Using the FRET pair Clover/mRuby2, we set up a flow cytometry-based FRET assay by analyzing PPARγ1 binding to its heterodimerization partner RXRα. Analyses of PPARγ-reporter and co-localization studies by laser-scanning microscopy validated this system. Refining the system, we created a new readout to distinguish strong from weak interactions, focusing on PPARγ-binding to the co-repressor N-CoR2. Results: We observed high FRET in cells expressing Clover-PPARγ1 and mRuby2-RXRα, but no FRET when cells express a mRuby2-RXRα deletion mutant, lacking the PPARγ interaction domain. Focusing on the co-repressor N-CoR2, we identified in HEK293T cells the new splice variant N-CoR2-ΔID1-exon. Overexpressing this isoform tagged with mRuby2, revealed no binding to Clover-PPARγ1, nor in murine J774A.1 macrophages. In HEK293T cells, binding was even lower in comparison to N-CoR2 constructs in which domains established to mediate interaction with PPARγ binding are deleted. These data suggest a possible role of N-CoR2-ΔID1-exon as a dominant negative variant. Because binding to N-CoR2-mRuby2 was not altered following activation or antagonism of Clover-PPARγ1, we determined the effect of pharmacological treatment on FRET intensity. Therefore, we calculated flow cytometry-based FRET efficiencies based on our flow cytometry data. As with PPARγ antagonism, PPARγ agonist treatment did not prevent binding of N-CoR2. Conclusion: Our system allows the close determination of protein-protein interactions with a special focus on binding intensity, allowing this system to characterize the role of protein domains as well as the effect of pharmacological agents on protein-protein interactions.
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spelling pubmed-67353822019-09-18 Flow cytometry-based FRET identifies binding intensities in PPARγ1 protein-protein interactions in living cells Trümper, Verena von Knethen, Andreas Preuß, Annegret Ermilov, Eugeny Hackbarth, Steffen Kuchler, Laura Gunne, Sandra Schäfer, Anne Bornhütter, Tobias Vereb, György Ujlaky-Nagy, Lázló Brüne, Bernhard Röder, Beate Schindler, Michael Parnham, Michael J. Knape, Tilo Theranostics Research Paper PPARγ is a pharmacological target in inflammatory and metabolic diseases. Upon agonistic treatment or following antagonism, binding of co-factors is altered, which consequently affects PPARγ-dependent transactivation as well as its DNA-independent properties. Therefore, establishing techniques to characterize these interactions is an important issue in living cells. Methods: Using the FRET pair Clover/mRuby2, we set up a flow cytometry-based FRET assay by analyzing PPARγ1 binding to its heterodimerization partner RXRα. Analyses of PPARγ-reporter and co-localization studies by laser-scanning microscopy validated this system. Refining the system, we created a new readout to distinguish strong from weak interactions, focusing on PPARγ-binding to the co-repressor N-CoR2. Results: We observed high FRET in cells expressing Clover-PPARγ1 and mRuby2-RXRα, but no FRET when cells express a mRuby2-RXRα deletion mutant, lacking the PPARγ interaction domain. Focusing on the co-repressor N-CoR2, we identified in HEK293T cells the new splice variant N-CoR2-ΔID1-exon. Overexpressing this isoform tagged with mRuby2, revealed no binding to Clover-PPARγ1, nor in murine J774A.1 macrophages. In HEK293T cells, binding was even lower in comparison to N-CoR2 constructs in which domains established to mediate interaction with PPARγ binding are deleted. These data suggest a possible role of N-CoR2-ΔID1-exon as a dominant negative variant. Because binding to N-CoR2-mRuby2 was not altered following activation or antagonism of Clover-PPARγ1, we determined the effect of pharmacological treatment on FRET intensity. Therefore, we calculated flow cytometry-based FRET efficiencies based on our flow cytometry data. As with PPARγ antagonism, PPARγ agonist treatment did not prevent binding of N-CoR2. Conclusion: Our system allows the close determination of protein-protein interactions with a special focus on binding intensity, allowing this system to characterize the role of protein domains as well as the effect of pharmacological agents on protein-protein interactions. Ivyspring International Publisher 2019-07-28 /pmc/articles/PMC6735382/ /pubmed/31534496 http://dx.doi.org/10.7150/thno.29367 Text en © The author(s) This is an open access article distributed under the terms of the Creative Commons Attribution License (https://creativecommons.org/licenses/by/4.0/). See http://ivyspring.com/terms for full terms and conditions.
spellingShingle Research Paper
Trümper, Verena
von Knethen, Andreas
Preuß, Annegret
Ermilov, Eugeny
Hackbarth, Steffen
Kuchler, Laura
Gunne, Sandra
Schäfer, Anne
Bornhütter, Tobias
Vereb, György
Ujlaky-Nagy, Lázló
Brüne, Bernhard
Röder, Beate
Schindler, Michael
Parnham, Michael J.
Knape, Tilo
Flow cytometry-based FRET identifies binding intensities in PPARγ1 protein-protein interactions in living cells
title Flow cytometry-based FRET identifies binding intensities in PPARγ1 protein-protein interactions in living cells
title_full Flow cytometry-based FRET identifies binding intensities in PPARγ1 protein-protein interactions in living cells
title_fullStr Flow cytometry-based FRET identifies binding intensities in PPARγ1 protein-protein interactions in living cells
title_full_unstemmed Flow cytometry-based FRET identifies binding intensities in PPARγ1 protein-protein interactions in living cells
title_short Flow cytometry-based FRET identifies binding intensities in PPARγ1 protein-protein interactions in living cells
title_sort flow cytometry-based fret identifies binding intensities in pparγ1 protein-protein interactions in living cells
topic Research Paper
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6735382/
https://www.ncbi.nlm.nih.gov/pubmed/31534496
http://dx.doi.org/10.7150/thno.29367
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