An Automated High-Throughput Cell-Based Multiplexed Flow Cytometry Assay to Identify Novel Compounds to Target Candida albicans Virulence-Related Proteins

Although three major classes of systemic antifungal agents are clinically available, each is characterized by important limitations. Thus, there has been considerable ongoing effort to develop novel and repurposed agents for the therapy of invasive fungal infections. In an effort to address these ne...

Descripción completa

Detalles Bibliográficos
Autores principales: Bernardo, Stella M., Allen, Christopher P., Waller, Anna, Young, Susan M., Oprea, Tudor, Sklar, Larry A., Lee, Samuel A.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2014
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4211665/
https://www.ncbi.nlm.nih.gov/pubmed/25350399
http://dx.doi.org/10.1371/journal.pone.0110354
_version_ 1782341606692618240
author Bernardo, Stella M.
Allen, Christopher P.
Waller, Anna
Young, Susan M.
Oprea, Tudor
Sklar, Larry A.
Lee, Samuel A.
author_facet Bernardo, Stella M.
Allen, Christopher P.
Waller, Anna
Young, Susan M.
Oprea, Tudor
Sklar, Larry A.
Lee, Samuel A.
author_sort Bernardo, Stella M.
collection PubMed
description Although three major classes of systemic antifungal agents are clinically available, each is characterized by important limitations. Thus, there has been considerable ongoing effort to develop novel and repurposed agents for the therapy of invasive fungal infections. In an effort to address these needs, we developed a novel high-throughput, multiplexed screening method that utilizes small molecules to probe candidate drug targets in the opportunistic fungal pathogen Candida albicans. This method is amenable to high-throughput automated screening and is based upon detection of changes in GFP levels of individually tagged target proteins. We first selected four GFP-tagged membrane-bound proteins associated with virulence or antifungal drug resistance in C. albicans. We demonstrated proof-of-principle that modulation of fluorescence intensity can be used to assay the expression of specific GFP-tagged target proteins to inhibitors (and inducers), and this change is measurable within the HyperCyt automated flow cytometry sampling system. Next, we generated a multiplex of differentially color-coded C. albicans strains bearing C-terminal GFP-tags of each gene encoding candidate drug targets incubated in the presence of small molecules from the Prestwick Chemical Library in 384-well microtiter plate format. Following incubation, cells were sampled through the HyperCyt system and modulation of protein levels, as indicated by changes in GFP-levels of each strain, was used to identify compounds of interest. The hit rate for both inducers and inhibitors identified in the primary screen did not exceed 1% of the total number of compounds in the small-molecule library that was probed, as would be expected from a robust target-specific, high-throughput screening campaign. Secondary assays for virulence characteristics based on null mutant strains were then used to further validate specificity. In all, this study presents a method for the identification and verification of new antifungal drugs targeted to fungal virulence proteins using C. albicans as a model fungal pathogen.
format Online
Article
Text
id pubmed-4211665
institution National Center for Biotechnology Information
language English
publishDate 2014
publisher Public Library of Science
record_format MEDLINE/PubMed
spelling pubmed-42116652014-11-05 An Automated High-Throughput Cell-Based Multiplexed Flow Cytometry Assay to Identify Novel Compounds to Target Candida albicans Virulence-Related Proteins Bernardo, Stella M. Allen, Christopher P. Waller, Anna Young, Susan M. Oprea, Tudor Sklar, Larry A. Lee, Samuel A. PLoS One Research Article Although three major classes of systemic antifungal agents are clinically available, each is characterized by important limitations. Thus, there has been considerable ongoing effort to develop novel and repurposed agents for the therapy of invasive fungal infections. In an effort to address these needs, we developed a novel high-throughput, multiplexed screening method that utilizes small molecules to probe candidate drug targets in the opportunistic fungal pathogen Candida albicans. This method is amenable to high-throughput automated screening and is based upon detection of changes in GFP levels of individually tagged target proteins. We first selected four GFP-tagged membrane-bound proteins associated with virulence or antifungal drug resistance in C. albicans. We demonstrated proof-of-principle that modulation of fluorescence intensity can be used to assay the expression of specific GFP-tagged target proteins to inhibitors (and inducers), and this change is measurable within the HyperCyt automated flow cytometry sampling system. Next, we generated a multiplex of differentially color-coded C. albicans strains bearing C-terminal GFP-tags of each gene encoding candidate drug targets incubated in the presence of small molecules from the Prestwick Chemical Library in 384-well microtiter plate format. Following incubation, cells were sampled through the HyperCyt system and modulation of protein levels, as indicated by changes in GFP-levels of each strain, was used to identify compounds of interest. The hit rate for both inducers and inhibitors identified in the primary screen did not exceed 1% of the total number of compounds in the small-molecule library that was probed, as would be expected from a robust target-specific, high-throughput screening campaign. Secondary assays for virulence characteristics based on null mutant strains were then used to further validate specificity. In all, this study presents a method for the identification and verification of new antifungal drugs targeted to fungal virulence proteins using C. albicans as a model fungal pathogen. Public Library of Science 2014-10-28 /pmc/articles/PMC4211665/ /pubmed/25350399 http://dx.doi.org/10.1371/journal.pone.0110354 Text en https://creativecommons.org/publicdomain/zero/1.0/ This is an open-access article distributed under the terms of the Creative Commons Public Domain declaration, which stipulates that, once placed in the public domain, this work may be freely reproduced, distributed, transmitted, modified, built upon, or otherwise used by anyone for any lawful purpose.
spellingShingle Research Article
Bernardo, Stella M.
Allen, Christopher P.
Waller, Anna
Young, Susan M.
Oprea, Tudor
Sklar, Larry A.
Lee, Samuel A.
An Automated High-Throughput Cell-Based Multiplexed Flow Cytometry Assay to Identify Novel Compounds to Target Candida albicans Virulence-Related Proteins
title An Automated High-Throughput Cell-Based Multiplexed Flow Cytometry Assay to Identify Novel Compounds to Target Candida albicans Virulence-Related Proteins
title_full An Automated High-Throughput Cell-Based Multiplexed Flow Cytometry Assay to Identify Novel Compounds to Target Candida albicans Virulence-Related Proteins
title_fullStr An Automated High-Throughput Cell-Based Multiplexed Flow Cytometry Assay to Identify Novel Compounds to Target Candida albicans Virulence-Related Proteins
title_full_unstemmed An Automated High-Throughput Cell-Based Multiplexed Flow Cytometry Assay to Identify Novel Compounds to Target Candida albicans Virulence-Related Proteins
title_short An Automated High-Throughput Cell-Based Multiplexed Flow Cytometry Assay to Identify Novel Compounds to Target Candida albicans Virulence-Related Proteins
title_sort automated high-throughput cell-based multiplexed flow cytometry assay to identify novel compounds to target candida albicans virulence-related proteins
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4211665/
https://www.ncbi.nlm.nih.gov/pubmed/25350399
http://dx.doi.org/10.1371/journal.pone.0110354
work_keys_str_mv AT bernardostellam anautomatedhighthroughputcellbasedmultiplexedflowcytometryassaytoidentifynovelcompoundstotargetcandidaalbicansvirulencerelatedproteins
AT allenchristopherp anautomatedhighthroughputcellbasedmultiplexedflowcytometryassaytoidentifynovelcompoundstotargetcandidaalbicansvirulencerelatedproteins
AT walleranna anautomatedhighthroughputcellbasedmultiplexedflowcytometryassaytoidentifynovelcompoundstotargetcandidaalbicansvirulencerelatedproteins
AT youngsusanm anautomatedhighthroughputcellbasedmultiplexedflowcytometryassaytoidentifynovelcompoundstotargetcandidaalbicansvirulencerelatedproteins
AT opreatudor anautomatedhighthroughputcellbasedmultiplexedflowcytometryassaytoidentifynovelcompoundstotargetcandidaalbicansvirulencerelatedproteins
AT sklarlarrya anautomatedhighthroughputcellbasedmultiplexedflowcytometryassaytoidentifynovelcompoundstotargetcandidaalbicansvirulencerelatedproteins
AT leesamuela anautomatedhighthroughputcellbasedmultiplexedflowcytometryassaytoidentifynovelcompoundstotargetcandidaalbicansvirulencerelatedproteins
AT bernardostellam automatedhighthroughputcellbasedmultiplexedflowcytometryassaytoidentifynovelcompoundstotargetcandidaalbicansvirulencerelatedproteins
AT allenchristopherp automatedhighthroughputcellbasedmultiplexedflowcytometryassaytoidentifynovelcompoundstotargetcandidaalbicansvirulencerelatedproteins
AT walleranna automatedhighthroughputcellbasedmultiplexedflowcytometryassaytoidentifynovelcompoundstotargetcandidaalbicansvirulencerelatedproteins
AT youngsusanm automatedhighthroughputcellbasedmultiplexedflowcytometryassaytoidentifynovelcompoundstotargetcandidaalbicansvirulencerelatedproteins
AT opreatudor automatedhighthroughputcellbasedmultiplexedflowcytometryassaytoidentifynovelcompoundstotargetcandidaalbicansvirulencerelatedproteins
AT sklarlarrya automatedhighthroughputcellbasedmultiplexedflowcytometryassaytoidentifynovelcompoundstotargetcandidaalbicansvirulencerelatedproteins
AT leesamuela automatedhighthroughputcellbasedmultiplexedflowcytometryassaytoidentifynovelcompoundstotargetcandidaalbicansvirulencerelatedproteins

Ejemplares similares