Development of a cell-free split-luciferase biochemical assay as a tool for screening for inhibitors of challenging protein-protein interaction targets

Targeting the interaction of proteins with weak binding affinities or low solubility represents a particular challenge for drug screening. The NanoLuc (â )® Binary Technology (NanoBiT (â )®) was originally developed to detect protein-protein interactions in live mammalian cells. Here we report the s...

Descripción completa

Detalles Bibliográficos
Autores principales: Cooley, Rachel, Kara, Neesha, Hui, Ning Sze, Tart, Jonathan, Roustan, Chloë, George, Roger, Hancock, David C., Binkowski, Brock F., Wood, Keith V., Ismail, Mohamed, Downward, Julian
Formato: Online Artículo Texto
Lenguaje:English
Publicado: F1000 Research Limited 2020
Materias:
Method Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7308888/
https://www.ncbi.nlm.nih.gov/pubmed/32587898
http://dx.doi.org/10.12688/wellcomeopenres.15675.1
_version_ 1783549096679702528
author Cooley, Rachel
Kara, Neesha
Hui, Ning Sze
Tart, Jonathan
Roustan, Chloë
George, Roger
Hancock, David C.
Binkowski, Brock F.
Wood, Keith V.
Ismail, Mohamed
Downward, Julian
author_facet Cooley, Rachel
Kara, Neesha
Hui, Ning Sze
Tart, Jonathan
Roustan, Chloë
George, Roger
Hancock, David C.
Binkowski, Brock F.
Wood, Keith V.
Ismail, Mohamed
Downward, Julian
author_sort Cooley, Rachel
collection PubMed
description Targeting the interaction of proteins with weak binding affinities or low solubility represents a particular challenge for drug screening. The NanoLuc (â )® Binary Technology (NanoBiT (â )®) was originally developed to detect protein-protein interactions in live mammalian cells. Here we report the successful translation of the NanoBit cellular assay into a biochemical, cell-free format using mammalian cell lysates. We show that the assay is suitable for the detection of both strong and weak protein interactions such as those involving the binding of RAS oncoproteins to either RAF or phosphoinositide 3-kinase (PI3K) effectors respectively, and that it is also effective for the study of poorly soluble protein domains such as the RAS binding domain of PI3K. Furthermore, the RAS interaction assay is sensitive and responds to both strong and weak RAS inhibitors. Our data show that the assay is robust, reproducible, cost-effective, and can be adapted for small and large-scale screening approaches. The NanoBit Biochemical Assay offers an attractive tool for drug screening against challenging protein-protein interaction targets, including the interaction of RAS with PI3K.
format Online
Article
Text
id pubmed-7308888
institution National Center for Biotechnology Information
language English
publishDate 2020
publisher F1000 Research Limited
record_format MEDLINE/PubMed
spelling pubmed-73088882020-06-24 Development of a cell-free split-luciferase biochemical assay as a tool for screening for inhibitors of challenging protein-protein interaction targets Cooley, Rachel Kara, Neesha Hui, Ning Sze Tart, Jonathan Roustan, Chloë George, Roger Hancock, David C. Binkowski, Brock F. Wood, Keith V. Ismail, Mohamed Downward, Julian Wellcome Open Res Method Article Targeting the interaction of proteins with weak binding affinities or low solubility represents a particular challenge for drug screening. The NanoLuc (â )® Binary Technology (NanoBiT (â )®) was originally developed to detect protein-protein interactions in live mammalian cells. Here we report the successful translation of the NanoBit cellular assay into a biochemical, cell-free format using mammalian cell lysates. We show that the assay is suitable for the detection of both strong and weak protein interactions such as those involving the binding of RAS oncoproteins to either RAF or phosphoinositide 3-kinase (PI3K) effectors respectively, and that it is also effective for the study of poorly soluble protein domains such as the RAS binding domain of PI3K. Furthermore, the RAS interaction assay is sensitive and responds to both strong and weak RAS inhibitors. Our data show that the assay is robust, reproducible, cost-effective, and can be adapted for small and large-scale screening approaches. The NanoBit Biochemical Assay offers an attractive tool for drug screening against challenging protein-protein interaction targets, including the interaction of RAS with PI3K. F1000 Research Limited 2020-02-06 /pmc/articles/PMC7308888/ /pubmed/32587898 http://dx.doi.org/10.12688/wellcomeopenres.15675.1 Text en Copyright: © 2020 Cooley R et al. http://creativecommons.org/licenses/by/4.0/ This is an open access article distributed under the terms of the Creative Commons Attribution Licence, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Method Article
Cooley, Rachel
Kara, Neesha
Hui, Ning Sze
Tart, Jonathan
Roustan, Chloë
George, Roger
Hancock, David C.
Binkowski, Brock F.
Wood, Keith V.
Ismail, Mohamed
Downward, Julian
Development of a cell-free split-luciferase biochemical assay as a tool for screening for inhibitors of challenging protein-protein interaction targets
title Development of a cell-free split-luciferase biochemical assay as a tool for screening for inhibitors of challenging protein-protein interaction targets
title_full Development of a cell-free split-luciferase biochemical assay as a tool for screening for inhibitors of challenging protein-protein interaction targets
title_fullStr Development of a cell-free split-luciferase biochemical assay as a tool for screening for inhibitors of challenging protein-protein interaction targets
title_full_unstemmed Development of a cell-free split-luciferase biochemical assay as a tool for screening for inhibitors of challenging protein-protein interaction targets
title_short Development of a cell-free split-luciferase biochemical assay as a tool for screening for inhibitors of challenging protein-protein interaction targets
title_sort development of a cell-free split-luciferase biochemical assay as a tool for screening for inhibitors of challenging protein-protein interaction targets
topic Method Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7308888/
https://www.ncbi.nlm.nih.gov/pubmed/32587898
http://dx.doi.org/10.12688/wellcomeopenres.15675.1
work_keys_str_mv AT cooleyrachel developmentofacellfreesplitluciferasebiochemicalassayasatoolforscreeningforinhibitorsofchallengingproteinproteininteractiontargets
AT karaneesha developmentofacellfreesplitluciferasebiochemicalassayasatoolforscreeningforinhibitorsofchallengingproteinproteininteractiontargets
AT huiningsze developmentofacellfreesplitluciferasebiochemicalassayasatoolforscreeningforinhibitorsofchallengingproteinproteininteractiontargets
AT tartjonathan developmentofacellfreesplitluciferasebiochemicalassayasatoolforscreeningforinhibitorsofchallengingproteinproteininteractiontargets
AT roustanchloe developmentofacellfreesplitluciferasebiochemicalassayasatoolforscreeningforinhibitorsofchallengingproteinproteininteractiontargets
AT georgeroger developmentofacellfreesplitluciferasebiochemicalassayasatoolforscreeningforinhibitorsofchallengingproteinproteininteractiontargets
AT hancockdavidc developmentofacellfreesplitluciferasebiochemicalassayasatoolforscreeningforinhibitorsofchallengingproteinproteininteractiontargets
AT binkowskibrockf developmentofacellfreesplitluciferasebiochemicalassayasatoolforscreeningforinhibitorsofchallengingproteinproteininteractiontargets
AT woodkeithv developmentofacellfreesplitluciferasebiochemicalassayasatoolforscreeningforinhibitorsofchallengingproteinproteininteractiontargets
AT ismailmohamed developmentofacellfreesplitluciferasebiochemicalassayasatoolforscreeningforinhibitorsofchallengingproteinproteininteractiontargets
AT downwardjulian developmentofacellfreesplitluciferasebiochemicalassayasatoolforscreeningforinhibitorsofchallengingproteinproteininteractiontargets

Ejemplares similares