Development of a fluorescence-based cellular apoptosis reporter

Lucy A. Balderstone; John Dawson; Arkadiusz Welman; Alan Serrels; Stephen R. Wedge; Valerie Brunton

doi:10.1088/2050-6120/aae6f8

Development of a fluorescence-based cellular apoptosis reporter

Lucy A. Balderstone, John Dawson, Arkadiusz Welman, Alan Serrels, Stephen R. Wedge, Valerie Brunton

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

Abstract

Evasion of apoptosis is a hallmark of human cancer, and a desired endpoint of many anticancer agents is the induction of cell death. With the heterogeneity of cancer becoming increasingly apparent, to understand drug mechanisms of action and identify combination therapies in cell populations, the development of tools to assess drug effects at the single cell level is a necessity for future preclinical drug development. Herein we describe the development of pCasFSwitch, a genetically encoded reporter construct designed to identify cells undergoing caspase-3 mediated apoptosis, by a translocation of a GFP signal from the cell membrane into the nucleus. Anticipated cellular distribution was demonstrated by use of confocal microscopy and cleavage by caspase-3 was shown to be required for the translocation of the GFP signal seen in apoptotic cells. Quantification of apoptosis using the construct revealed similar levels
to that obtained with a commercially available apoptosis imaging agent (22.6 % versus 20.3%). Moreover, we demonstrated its capacity for use in a high-throughput setting making it a powerful tool for drug development pipelines.

Original language	English
Journal	Methods and Applications in Fluorescence
Early online date	10 Oct 2018
DOIs	https://doi.org/10.1088/2050-6120/aae6f8
Publication status	Published - 24 Oct 2018

Keywords / Materials (for Non-textual outputs)

apoptosis
caspase
fluorescence

Access to Document

10.1088/2050-6120/aae6f8Licence: Creative Commons: Attribution (CC-BY)

2018.10.09 Published AAM Development of a fluorescence based cellular apoptosis reporter
As the Version of Record of this article is going to be / has been published on a gold open access basis under a CC BY 3.0 licence, this Accepted Manuscript is available for reuse under a CC BY 3.0 licence immediately
Accepted author manuscript, 6.43 MBLicence: Creative Commons: Attribution (CC-BY)
2018 Oct 24 Development of a fluorescence - based cellular apoptosis reporterFinal published version, 1.54 MBLicence: CC BY

Cancer Research UK Edinburgh Centre Award 2017/2018
Frame, M. (Principal Investigator) & Tomlinson, I. (Co-investigator)
UK-based charities
1/04/17 → 31/03/22
Project: Research

Cite this

@article{e483e68d2b4b4f988090af65d475ef74,

title = "Development of a fluorescence-based cellular apoptosis reporter",

abstract = "Evasion of apoptosis is a hallmark of human cancer, and a desired endpoint of many anticancer agents is the induction of cell death. With the heterogeneity of cancer becoming increasingly apparent, to understand drug mechanisms of action and identify combination therapies in cell populations, the development of tools to assess drug effects at the single cell level is a necessity for future preclinical drug development. Herein we describe the development of pCasFSwitch, a genetically encoded reporter construct designed to identify cells undergoing caspase-3 mediated apoptosis, by a translocation of a GFP signal from the cell membrane into the nucleus. Anticipated cellular distribution was demonstrated by use of confocal microscopy and cleavage by caspase-3 was shown to be required for the translocation of the GFP signal seen in apoptotic cells. Quantification of apoptosis using the construct revealed similar levelsto that obtained with a commercially available apoptosis imaging agent (22.6 % versus 20.3%). Moreover, we demonstrated its capacity for use in a high-throughput setting making it a powerful tool for drug development pipelines.",

keywords = "apoptosis, caspase, fluorescence",

author = "Balderstone, {Lucy A.} and John Dawson and Arkadiusz Welman and Alan Serrels and Wedge, {Stephen R.} and Valerie Brunton",

year = "2018",

month = oct,

day = "24",

doi = "10.1088/2050-6120/aae6f8",

language = "English",

journal = "Methods and Applications in Fluorescence",

issn = "2050-6120",

publisher = "IOP Publishing Ltd.",

}

TY - JOUR

T1 - Development of a fluorescence-based cellular apoptosis reporter

AU - Balderstone, Lucy A.

AU - Dawson, John

AU - Welman, Arkadiusz

AU - Serrels, Alan

AU - Wedge, Stephen R.

AU - Brunton, Valerie

PY - 2018/10/24

Y1 - 2018/10/24

N2 - Evasion of apoptosis is a hallmark of human cancer, and a desired endpoint of many anticancer agents is the induction of cell death. With the heterogeneity of cancer becoming increasingly apparent, to understand drug mechanisms of action and identify combination therapies in cell populations, the development of tools to assess drug effects at the single cell level is a necessity for future preclinical drug development. Herein we describe the development of pCasFSwitch, a genetically encoded reporter construct designed to identify cells undergoing caspase-3 mediated apoptosis, by a translocation of a GFP signal from the cell membrane into the nucleus. Anticipated cellular distribution was demonstrated by use of confocal microscopy and cleavage by caspase-3 was shown to be required for the translocation of the GFP signal seen in apoptotic cells. Quantification of apoptosis using the construct revealed similar levelsto that obtained with a commercially available apoptosis imaging agent (22.6 % versus 20.3%). Moreover, we demonstrated its capacity for use in a high-throughput setting making it a powerful tool for drug development pipelines.

AB - Evasion of apoptosis is a hallmark of human cancer, and a desired endpoint of many anticancer agents is the induction of cell death. With the heterogeneity of cancer becoming increasingly apparent, to understand drug mechanisms of action and identify combination therapies in cell populations, the development of tools to assess drug effects at the single cell level is a necessity for future preclinical drug development. Herein we describe the development of pCasFSwitch, a genetically encoded reporter construct designed to identify cells undergoing caspase-3 mediated apoptosis, by a translocation of a GFP signal from the cell membrane into the nucleus. Anticipated cellular distribution was demonstrated by use of confocal microscopy and cleavage by caspase-3 was shown to be required for the translocation of the GFP signal seen in apoptotic cells. Quantification of apoptosis using the construct revealed similar levelsto that obtained with a commercially available apoptosis imaging agent (22.6 % versus 20.3%). Moreover, we demonstrated its capacity for use in a high-throughput setting making it a powerful tool for drug development pipelines.

KW - apoptosis

KW - caspase

KW - fluorescence

U2 - 10.1088/2050-6120/aae6f8

DO - 10.1088/2050-6120/aae6f8

M3 - Article

SN - 2050-6120

JO - Methods and Applications in Fluorescence

JF - Methods and Applications in Fluorescence

ER -

Development of a fluorescence-based cellular apoptosis reporter

Abstract

Keywords / Materials (for Non-textual outputs)

Access to Document

Fingerprint

Projects

Cancer Research UK Edinburgh Centre Award 2017/2018

Cite this