A multi-biomarker micronucleus assay using imaging flow cytometry

Danielle S.G. Harte; Anthony M. Lynch; Jatin Verma; Paul Rees; Andrew Filby; John W. Wills; George E. Johnson

doi:10.1007/s00204-024-03801-7

A multi-biomarker micronucleus assay using imaging flow cytometry

Danielle S.G. Harte, Anthony M. Lynch, Jatin Verma, Paul Rees, Andrew Filby, John W. Wills, George E. Johnson

Research output: Contribution to journal › Article › peer-review

2 Scopus citations

Abstract

Genetic toxicity testing assesses the potential of compounds to cause DNA damage. There are many genetic toxicology screening assays designed to assess the DNA damaging potential of chemicals in early drug development aiding the identification of promising drugs that have low-risk potential for causing genetic damage contributing to cancer risk in humans. Despite this, in vitro tests generate a high number of misleading positives, the consequences of which can lead to unnecessary animal testing and/or the abandonment of promising drug candidates. Understanding chemical Mode of Action (MoA) is vital to identifying the true genotoxic potential of substances and, therefore, the risk translation into the clinic. Here we demonstrate a simple, robust protocol for staining fixed, human-lymphoblast p53 proficient TK6 cells with antibodies against ɣH2AX, p53 and pH3S28 along with DRAQ5™ DNA staining that enables analysis of un-lysed cells via microscopy approaches such as imaging flow cytometry. Here, we used the Cytek® Amnis® ImageStream®X Mk II which provides a high-throughput acquisition platform with the sensitivity of flow cytometry and spatial morphological information associated with microscopy. Using the ImageStream manufacturer’s software (IDEAS® 6.2), a masking strategy was developed to automatically detect and quantify micronucleus events (MN) and characterise biomarker populations. The gating strategy developed enables the generation of a template capable of automatically batch processing data files quantifying cell-cycle, MN, ɣH2AX, p53 and pH3 populations simultaneously. In this way, we demonstrate how a multiplex system enables DNA damage assessment alongside MN identification using un-lysed cells on the imaging flow cytometry platform. As a proof-of-concept, we use the tool chemicals carbendazim and methyl methanesulphonate (MMS) to demonstrate the assay’s ability to correctly identify clastogenic or aneugenic MoAs using the biomarker profiles established.

Original language	English (US)
Pages (from-to)	3137-3153
Number of pages	17
Journal	Archives of Toxicology
Volume	98
Issue number	9
DOIs	https://doi.org/10.1007/s00204-024-03801-7
State	Published - Sep 2024

Keywords

Biomarker
DNA damage
ImageStream
Micronucleus
MoA
NAM
Micronucleus Tests/methods
Cell Line
Image Cytometry/methods
Humans
Flow Cytometry/methods
Tumor Suppressor Protein p53/metabolism
Biomarkers/metabolism
Histones/metabolism
DNA Damage
Mutagens/toxicity

ASJC Scopus subject areas

Toxicology
Health, Toxicology and Mutagenesis

Access to Document

10.1007/s00204-024-03801-7

Cite this

@article{50ff2c9fe4fa454ab84f8b6757065d4a,

title = "A multi-biomarker micronucleus assay using imaging flow cytometry",

abstract = "Genetic toxicity testing assesses the potential of compounds to cause DNA damage. There are many genetic toxicology screening assays designed to assess the DNA damaging potential of chemicals in early drug development aiding the identification of promising drugs that have low-risk potential for causing genetic damage contributing to cancer risk in humans. Despite this, in vitro tests generate a high number of misleading positives, the consequences of which can lead to unnecessary animal testing and/or the abandonment of promising drug candidates. Understanding chemical Mode of Action (MoA) is vital to identifying the true genotoxic potential of substances and, therefore, the risk translation into the clinic. Here we demonstrate a simple, robust protocol for staining fixed, human-lymphoblast p53 proficient TK6 cells with antibodies against ɣH2AX, p53 and pH3S28 along with DRAQ5{\texttrademark} DNA staining that enables analysis of un-lysed cells via microscopy approaches such as imaging flow cytometry. Here, we used the Cytek{\textregistered} Amnis{\textregistered} ImageStream{\textregistered}X Mk II which provides a high-throughput acquisition platform with the sensitivity of flow cytometry and spatial morphological information associated with microscopy. Using the ImageStream manufacturer{\textquoteright}s software (IDEAS{\textregistered} 6.2), a masking strategy was developed to automatically detect and quantify micronucleus events (MN) and characterise biomarker populations. The gating strategy developed enables the generation of a template capable of automatically batch processing data files quantifying cell-cycle, MN, ɣH2AX, p53 and pH3 populations simultaneously. In this way, we demonstrate how a multiplex system enables DNA damage assessment alongside MN identification using un-lysed cells on the imaging flow cytometry platform. As a proof-of-concept, we use the tool chemicals carbendazim and methyl methanesulphonate (MMS) to demonstrate the assay{\textquoteright}s ability to correctly identify clastogenic or aneugenic MoAs using the biomarker profiles established.",

keywords = "Biomarker, DNA damage, ImageStream, Micronucleus, MoA, NAM, Micronucleus Tests/methods, Cell Line, Image Cytometry/methods, Humans, Flow Cytometry/methods, Tumor Suppressor Protein p53/metabolism, Biomarkers/metabolism, Histones/metabolism, DNA Damage, Mutagens/toxicity",

author = "Harte, \{Danielle S.G.\} and Lynch, \{Anthony M.\} and Jatin Verma and Paul Rees and Andrew Filby and Wills, \{John W.\} and Johnson, \{George E.\}",

note = "Publisher Copyright: {\textcopyright} The Author(s) 2024.",

year = "2024",

month = sep,

doi = "10.1007/s00204-024-03801-7",

language = "English (US)",

volume = "98",

pages = "3137--3153",

journal = "Archives of Toxicology",

issn = "0340-5761",

publisher = "Springer Science and Business Media Deutschland GmbH",

number = "9",

}

TY - JOUR

T1 - A multi-biomarker micronucleus assay using imaging flow cytometry

AU - Harte, Danielle S.G.

AU - Lynch, Anthony M.

AU - Verma, Jatin

AU - Rees, Paul

AU - Filby, Andrew

AU - Wills, John W.

AU - Johnson, George E.

N1 - Publisher Copyright: © The Author(s) 2024.

PY - 2024/9

Y1 - 2024/9

N2 - Genetic toxicity testing assesses the potential of compounds to cause DNA damage. There are many genetic toxicology screening assays designed to assess the DNA damaging potential of chemicals in early drug development aiding the identification of promising drugs that have low-risk potential for causing genetic damage contributing to cancer risk in humans. Despite this, in vitro tests generate a high number of misleading positives, the consequences of which can lead to unnecessary animal testing and/or the abandonment of promising drug candidates. Understanding chemical Mode of Action (MoA) is vital to identifying the true genotoxic potential of substances and, therefore, the risk translation into the clinic. Here we demonstrate a simple, robust protocol for staining fixed, human-lymphoblast p53 proficient TK6 cells with antibodies against ɣH2AX, p53 and pH3S28 along with DRAQ5™ DNA staining that enables analysis of un-lysed cells via microscopy approaches such as imaging flow cytometry. Here, we used the Cytek® Amnis® ImageStream®X Mk II which provides a high-throughput acquisition platform with the sensitivity of flow cytometry and spatial morphological information associated with microscopy. Using the ImageStream manufacturer’s software (IDEAS® 6.2), a masking strategy was developed to automatically detect and quantify micronucleus events (MN) and characterise biomarker populations. The gating strategy developed enables the generation of a template capable of automatically batch processing data files quantifying cell-cycle, MN, ɣH2AX, p53 and pH3 populations simultaneously. In this way, we demonstrate how a multiplex system enables DNA damage assessment alongside MN identification using un-lysed cells on the imaging flow cytometry platform. As a proof-of-concept, we use the tool chemicals carbendazim and methyl methanesulphonate (MMS) to demonstrate the assay’s ability to correctly identify clastogenic or aneugenic MoAs using the biomarker profiles established.

AB - Genetic toxicity testing assesses the potential of compounds to cause DNA damage. There are many genetic toxicology screening assays designed to assess the DNA damaging potential of chemicals in early drug development aiding the identification of promising drugs that have low-risk potential for causing genetic damage contributing to cancer risk in humans. Despite this, in vitro tests generate a high number of misleading positives, the consequences of which can lead to unnecessary animal testing and/or the abandonment of promising drug candidates. Understanding chemical Mode of Action (MoA) is vital to identifying the true genotoxic potential of substances and, therefore, the risk translation into the clinic. Here we demonstrate a simple, robust protocol for staining fixed, human-lymphoblast p53 proficient TK6 cells with antibodies against ɣH2AX, p53 and pH3S28 along with DRAQ5™ DNA staining that enables analysis of un-lysed cells via microscopy approaches such as imaging flow cytometry. Here, we used the Cytek® Amnis® ImageStream®X Mk II which provides a high-throughput acquisition platform with the sensitivity of flow cytometry and spatial morphological information associated with microscopy. Using the ImageStream manufacturer’s software (IDEAS® 6.2), a masking strategy was developed to automatically detect and quantify micronucleus events (MN) and characterise biomarker populations. The gating strategy developed enables the generation of a template capable of automatically batch processing data files quantifying cell-cycle, MN, ɣH2AX, p53 and pH3 populations simultaneously. In this way, we demonstrate how a multiplex system enables DNA damage assessment alongside MN identification using un-lysed cells on the imaging flow cytometry platform. As a proof-of-concept, we use the tool chemicals carbendazim and methyl methanesulphonate (MMS) to demonstrate the assay’s ability to correctly identify clastogenic or aneugenic MoAs using the biomarker profiles established.

KW - Biomarker

KW - DNA damage

KW - ImageStream

KW - Micronucleus

KW - MoA

KW - NAM

KW - Micronucleus Tests/methods

KW - Cell Line

KW - Image Cytometry/methods

KW - Humans

KW - Flow Cytometry/methods

KW - Tumor Suppressor Protein p53/metabolism

KW - Biomarkers/metabolism

KW - Histones/metabolism

KW - DNA Damage

KW - Mutagens/toxicity

UR - https://www.scopus.com/pages/publications/85198552565

UR - https://www.scopus.com/inward/citedby.url?scp=85198552565&partnerID=8YFLogxK

U2 - 10.1007/s00204-024-03801-7

DO - 10.1007/s00204-024-03801-7

M3 - Article

C2 - 38995349

AN - SCOPUS:85198552565

SN - 0340-5761

VL - 98

SP - 3137

EP - 3153

JO - Archives of Toxicology

JF - Archives of Toxicology

IS - 9

ER -

A multi-biomarker micronucleus assay using imaging flow cytometry

Abstract

Keywords

ASJC Scopus subject areas

Access to Document

Other files and links

Fingerprint

Cite this