Correlation between luminescence intensity and cytotoxicity in cell-based cytotoxicity assay using luciferase

The luciferase reporter assay has become one of the conventional methods for cytotoxicity evaluation. Typically, the decrease of luminescence expressed by a constitutive promoter is used as an index of cytotoxicity. However, to our knowledge, there have been no reports of the correlation between cyt...

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Veröffentlicht in:	Analytical biochemistry 2017-04, Vol.522, p.18-29
Hauptverfasser:	Wakuri, S., Yamakage, K., Kazuki, Y., Kazuki, K., Oshimura, M., Aburatani, S., Yasunaga, M., Nakajima, Y.
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Schlagworte:	Animals Chromosomes, Artificial, Mammalian - genetics Chromosomes, Artificial, Mammalian - metabolism Coleoptera Cytotoxicity Hep G2 Cells Humans Insect Proteins - genetics Insect Proteins - metabolism Internal control reporter Luciferase Luciferase reporter assay Luciferases - genetics Luciferases - metabolism Luminescent Measurements - methods Mice Promoter Regions, Genetic Toxicity Tests - methods
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container_title	Analytical biochemistry
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creator	Wakuri, S. Yamakage, K. Kazuki, Y. Kazuki, K. Oshimura, M. Aburatani, S. Yasunaga, M. Nakajima, Y.
description	The luciferase reporter assay has become one of the conventional methods for cytotoxicity evaluation. Typically, the decrease of luminescence expressed by a constitutive promoter is used as an index of cytotoxicity. However, to our knowledge, there have been no reports of the correlation between cytotoxicity and luminescence intensity. In this study, to accurately verify the correlation between them, beetle luciferase was stably expressed in human hepatoma HepG2 cells harboring the multi-integrase mouse artificial chromosome vector. We showed that the cytotoxicity assay using luciferase does not depend on the stability of luciferase protein and the kind of constitutive promoter. Next, HepG2 cells in which green-emitting beetle luciferase was expressed under the control of CAG promoter were exposed to 58 compounds. The luminescence intensity and cytotoxicity curves of cells exposed to 48 compounds showed similar tendencies, whereas those of cells exposed to 10 compounds did not do so, although the curves gradually approached each other with increasing exposure time. Finally, we demonstrated that luciferase expressed under the control of a constitutive promoter can be utilized both as an internal control reporter for normalizing a test reporter and for monitoring cytotoxicity when two kinds of luciferases are simultaneously used in the cytotoxicity assay.
doi_str_mv	10.1016/j.ab.2017.01.015
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Typically, the decrease of luminescence expressed by a constitutive promoter is used as an index of cytotoxicity. However, to our knowledge, there have been no reports of the correlation between cytotoxicity and luminescence intensity. In this study, to accurately verify the correlation between them, beetle luciferase was stably expressed in human hepatoma HepG2 cells harboring the multi-integrase mouse artificial chromosome vector. We showed that the cytotoxicity assay using luciferase does not depend on the stability of luciferase protein and the kind of constitutive promoter. Next, HepG2 cells in which green-emitting beetle luciferase was expressed under the control of CAG promoter were exposed to 58 compounds. The luminescence intensity and cytotoxicity curves of cells exposed to 48 compounds showed similar tendencies, whereas those of cells exposed to 10 compounds did not do so, although the curves gradually approached each other with increasing exposure time. Finally, we demonstrated that luciferase expressed under the control of a constitutive promoter can be utilized both as an internal control reporter for normalizing a test reporter and for monitoring cytotoxicity when two kinds of luciferases are simultaneously used in the cytotoxicity assay.</description><identifier>ISSN: 0003-2697</identifier><identifier>EISSN: 1096-0309</identifier><identifier>DOI: 10.1016/j.ab.2017.01.015</identifier><identifier>PMID: 28111305</identifier><language>eng</language><publisher>United States: Elsevier Inc</publisher><subject>Animals ; Chromosomes, Artificial, Mammalian - genetics ; Chromosomes, Artificial, Mammalian - metabolism ; Coleoptera ; Cytotoxicity ; Hep G2 Cells ; Humans ; Insect Proteins - genetics ; Insect Proteins - metabolism ; Internal control reporter ; Luciferase ; Luciferase reporter assay ; Luciferases - genetics ; Luciferases - metabolism ; Luminescent Measurements - methods ; Mice ; Promoter Regions, Genetic ; Toxicity Tests - methods</subject><ispartof>Analytical biochemistry, 2017-04, Vol.522, p.18-29</ispartof><rights>2017 Elsevier Inc.</rights><rights>Copyright © 2017 Elsevier Inc. 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Typically, the decrease of luminescence expressed by a constitutive promoter is used as an index of cytotoxicity. However, to our knowledge, there have been no reports of the correlation between cytotoxicity and luminescence intensity. In this study, to accurately verify the correlation between them, beetle luciferase was stably expressed in human hepatoma HepG2 cells harboring the multi-integrase mouse artificial chromosome vector. We showed that the cytotoxicity assay using luciferase does not depend on the stability of luciferase protein and the kind of constitutive promoter. Next, HepG2 cells in which green-emitting beetle luciferase was expressed under the control of CAG promoter were exposed to 58 compounds. The luminescence intensity and cytotoxicity curves of cells exposed to 48 compounds showed similar tendencies, whereas those of cells exposed to 10 compounds did not do so, although the curves gradually approached each other with increasing exposure time. 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subjects	Animals Chromosomes, Artificial, Mammalian - genetics Chromosomes, Artificial, Mammalian - metabolism Coleoptera Cytotoxicity Hep G2 Cells Humans Insect Proteins - genetics Insect Proteins - metabolism Internal control reporter Luciferase Luciferase reporter assay Luciferases - genetics Luciferases - metabolism Luminescent Measurements - methods Mice Promoter Regions, Genetic Toxicity Tests - methods
title	Correlation between luminescence intensity and cytotoxicity in cell-based cytotoxicity assay using luciferase
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