Approved drugs screening against the nsP1 capping enzyme of Venezuelan equine encephalitis virus using an immuno-based assay

Ana S. Ferreira-Ramos; Changqing Li; Cécilia Eydoux; Jean Marie Contreras; Christophe Morice; Gilles Quérat; Alba Gigante; María Jesús Pérez Pérez; Marie Louise Jung; Bruno Canard; Jean Claude Guillemot; Etienne Decroly; Bruno Coutard

doi:10.1016/j.antiviral.2019.01.003

Approved drugs screening against the nsP1 capping enzyme of Venezuelan equine encephalitis virus using an immuno-based assay

Ana S. Ferreira-Ramos, Changqing Li, Cécilia Eydoux, Jean Marie Contreras, Christophe Morice, Gilles Quérat, Alba Gigante, María Jesús Pérez Pérez, Marie Louise Jung, Bruno Canard, Jean Claude Guillemot, Etienne Decroly, Bruno Coutard^*

^*Korrespondierende/r Autor/-in für diese Arbeit

Institut für Biochemie

Universität Aix-Marseille

17 Zitate (Scopus)

Abstract

Alphaviruses such as the Venezuelan equine encephalitis virus (VEEV) are important human emerging pathogens transmitted by mosquitoes. They possess a unique viral mRNA capping mechanism catalyzed by the viral non-structural protein nsP1, which is essential for virus replication. The alphaviruses capping starts by the methylation of a GTP molecule by the N7-guanine methyltransferase (MTase) activity; nsP1 then forms a covalent link with m ⁷ GMP releasing pyrophosphate (GT reaction) and the m ⁷ GMP is next transferred onto the 5′-diphosphate end of the viral mRNA to form a cap-0 structure. The cap-0 structure decreases the detection of foreign viral RNAs, prevents RNA degradation by cellular exonucleases, and promotes viral RNA translation into proteins. Additionally, reverse-genetic studies have demonstrated that viruses mutated in nsP1 catalytic residues are both impaired towards replication and attenuated. The nsP1 protein is thus considered an attractive antiviral target for drug discovery. We have previously demonstrated that the guanylylation of VEEV nsP1 can be monitored by Western blot analysis using an antibody recognizing the cap structure. In this study, we developed a high throughput ELISA screening assay to monitor the GT reaction through m ⁷ GMP-nsP1 adduct quantitation. This assay was validated using known nsP1 inhibitors before screening 1220 approved compounds. 18 compounds inhibiting the nsP1 guanylylation were identified, and their IC ₅₀ determined. Compounds from two series were further characterized and shown to inhibit the nsP1 MTase activity. Conversely, these compounds barely inhibited a cellular MTase demonstrating their specificity towards nsP1. Analogues search and SAR were also initiated to identify the active pharmacophore features. Altogether the results show that this HT enzyme-based assay is a convenient way to select potent and specific hit compounds targeting the viral mRNA capping of Alphaviruses.

Originalsprache	Englisch
Zeitschrift	Antiviral Research
Jahrgang	163
Seiten (von - bis)	59-69
Seitenumfang	11
ISSN	0166-3542
DOIs	https://doi.org/10.1016/j.antiviral.2019.01.003
Publikationsstatus	Veröffentlicht - 03.2019

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This work was supported by the French research agency ANR “VMTaseIn”, grant ANR-ST14-ASTR-0026 , and by the European Union ( Seventh Framework Program , Marie Skłodowska-Curie ETN “EUVIRNA”, grant agreement number 264286 and Horizon 2020 Marie Skłodowska-Curie ETN “ANTIVIRALS”, grant agreement number 642434 ), and by the MINECO/FEDER SAF2015-64629-C2-1-R . This work was supported by the French research agency ANR “VMTaseIn” grant ANR-ST14-ASTR-0026, and by the European Union (Seventh Framework Program, Marie Skłodowska-Curie ETN “EUVIRNA” grant agreement number 264286 and Horizon 2020 Marie Skłodowska-Curie ETN “ANTIVIRALS” grant agreement number 642434), and by the MINECO/FEDER SAF2015-64629-C2-1-R.

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Forschungsschwerpunkt: Infektion und Entzündung - Zentrum für Infektions- und Entzündungsforschung Lübeck (ZIEL)

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10.1016/j.antiviral.2019.01.003

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Ferreira-Ramos, A. S., Li, C., Eydoux, C., Contreras, J. M., Morice, C., Quérat, G., Gigante, A., Pérez Pérez, M. J., Jung, M. L., Canard, B., Guillemot, J. C., Decroly, E., & Coutard, B. (2019). Approved drugs screening against the nsP1 capping enzyme of Venezuelan equine encephalitis virus using an immuno-based assay. Antiviral Research, 163, 59-69. https://doi.org/10.1016/j.antiviral.2019.01.003

@article{e4a521a9704c4f20b066753bac579ed2,

title = "Approved drugs screening against the nsP1 capping enzyme of Venezuelan equine encephalitis virus using an immuno-based assay",

abstract = " Alphaviruses such as the Venezuelan equine encephalitis virus (VEEV) are important human emerging pathogens transmitted by mosquitoes. They possess a unique viral mRNA capping mechanism catalyzed by the viral non-structural protein nsP1, which is essential for virus replication. The alphaviruses capping starts by the methylation of a GTP molecule by the N7-guanine methyltransferase (MTase) activity; nsP1 then forms a covalent link with m 7 GMP releasing pyrophosphate (GT reaction) and the m 7 GMP is next transferred onto the 5′-diphosphate end of the viral mRNA to form a cap-0 structure. The cap-0 structure decreases the detection of foreign viral RNAs, prevents RNA degradation by cellular exonucleases, and promotes viral RNA translation into proteins. Additionally, reverse-genetic studies have demonstrated that viruses mutated in nsP1 catalytic residues are both impaired towards replication and attenuated. The nsP1 protein is thus considered an attractive antiviral target for drug discovery. We have previously demonstrated that the guanylylation of VEEV nsP1 can be monitored by Western blot analysis using an antibody recognizing the cap structure. In this study, we developed a high throughput ELISA screening assay to monitor the GT reaction through m 7 GMP-nsP1 adduct quantitation. This assay was validated using known nsP1 inhibitors before screening 1220 approved compounds. 18 compounds inhibiting the nsP1 guanylylation were identified, and their IC 50 determined. Compounds from two series were further characterized and shown to inhibit the nsP1 MTase activity. Conversely, these compounds barely inhibited a cellular MTase demonstrating their specificity towards nsP1. Analogues search and SAR were also initiated to identify the active pharmacophore features. Altogether the results show that this HT enzyme-based assay is a convenient way to select potent and specific hit compounds targeting the viral mRNA capping of Alphaviruses. ",

author = "Ferreira-Ramos, \{Ana S.\} and Changqing Li and C{\'e}cilia Eydoux and Contreras, \{Jean Marie\} and Christophe Morice and Gilles Qu{\'e}rat and Alba Gigante and \{P{\'e}rez P{\'e}rez\}, \{Mar{\'i}a Jes{\'u}s\} and Jung, \{Marie Louise\} and Bruno Canard and Guillemot, \{Jean Claude\} and Etienne Decroly and Bruno Coutard",

note = "Funding Information: This work was supported by the French research agency ANR “VMTaseIn”, grant ANR-ST14-ASTR-0026 , and by the European Union ( Seventh Framework Program , Marie Sk{\l}odowska-Curie ETN “EUVIRNA”, grant agreement number 264286 and Horizon 2020 Marie Sk{\l}odowska-Curie ETN “ANTIVIRALS”, grant agreement number 642434 ), and by the MINECO/FEDER SAF2015-64629-C2-1-R . Funding Information: This work was supported by the French research agency ANR “VMTaseIn” grant ANR-ST14-ASTR-0026, and by the European Union (Seventh Framework Program, Marie Sk{\l}odowska-Curie ETN “EUVIRNA” grant agreement number 264286 and Horizon 2020 Marie Sk{\l}odowska-Curie ETN “ANTIVIRALS” grant agreement number 642434), and by the MINECO/FEDER SAF2015-64629-C2-1-R. Publisher Copyright: {\textcopyright} 2019 Elsevier B.V. Copyright: Copyright 2019 Elsevier B.V., All rights reserved.",

year = "2019",

month = mar,

doi = "10.1016/j.antiviral.2019.01.003",

language = "English",

volume = "163",

pages = "59--69",

journal = "Antiviral Research",

issn = "0166-3542",

publisher = "Elsevier B.V.",

}

Ferreira-Ramos, AS, Li, C, Eydoux, C, Contreras, JM, Morice, C, Quérat, G, Gigante, A, Pérez Pérez, MJ, Jung, ML, Canard, B, Guillemot, JC, Decroly, E & Coutard, B 2019, 'Approved drugs screening against the nsP1 capping enzyme of Venezuelan equine encephalitis virus using an immuno-based assay', Antiviral Research, Jg. 163, S. 59-69. https://doi.org/10.1016/j.antiviral.2019.01.003

TY - JOUR

T1 - Approved drugs screening against the nsP1 capping enzyme of Venezuelan equine encephalitis virus using an immuno-based assay

AU - Ferreira-Ramos, Ana S.

AU - Li, Changqing

AU - Eydoux, Cécilia

AU - Contreras, Jean Marie

AU - Morice, Christophe

AU - Quérat, Gilles

AU - Gigante, Alba

AU - Pérez Pérez, María Jesús

AU - Jung, Marie Louise

AU - Canard, Bruno

AU - Guillemot, Jean Claude

AU - Decroly, Etienne

AU - Coutard, Bruno

N1 - Funding Information: This work was supported by the French research agency ANR “VMTaseIn”, grant ANR-ST14-ASTR-0026 , and by the European Union ( Seventh Framework Program , Marie Skłodowska-Curie ETN “EUVIRNA”, grant agreement number 264286 and Horizon 2020 Marie Skłodowska-Curie ETN “ANTIVIRALS”, grant agreement number 642434 ), and by the MINECO/FEDER SAF2015-64629-C2-1-R . Funding Information: This work was supported by the French research agency ANR “VMTaseIn” grant ANR-ST14-ASTR-0026, and by the European Union (Seventh Framework Program, Marie Skłodowska-Curie ETN “EUVIRNA” grant agreement number 264286 and Horizon 2020 Marie Skłodowska-Curie ETN “ANTIVIRALS” grant agreement number 642434), and by the MINECO/FEDER SAF2015-64629-C2-1-R. Publisher Copyright: © 2019 Elsevier B.V. Copyright: Copyright 2019 Elsevier B.V., All rights reserved.

PY - 2019/3

Y1 - 2019/3

N2 - Alphaviruses such as the Venezuelan equine encephalitis virus (VEEV) are important human emerging pathogens transmitted by mosquitoes. They possess a unique viral mRNA capping mechanism catalyzed by the viral non-structural protein nsP1, which is essential for virus replication. The alphaviruses capping starts by the methylation of a GTP molecule by the N7-guanine methyltransferase (MTase) activity; nsP1 then forms a covalent link with m 7 GMP releasing pyrophosphate (GT reaction) and the m 7 GMP is next transferred onto the 5′-diphosphate end of the viral mRNA to form a cap-0 structure. The cap-0 structure decreases the detection of foreign viral RNAs, prevents RNA degradation by cellular exonucleases, and promotes viral RNA translation into proteins. Additionally, reverse-genetic studies have demonstrated that viruses mutated in nsP1 catalytic residues are both impaired towards replication and attenuated. The nsP1 protein is thus considered an attractive antiviral target for drug discovery. We have previously demonstrated that the guanylylation of VEEV nsP1 can be monitored by Western blot analysis using an antibody recognizing the cap structure. In this study, we developed a high throughput ELISA screening assay to monitor the GT reaction through m 7 GMP-nsP1 adduct quantitation. This assay was validated using known nsP1 inhibitors before screening 1220 approved compounds. 18 compounds inhibiting the nsP1 guanylylation were identified, and their IC 50 determined. Compounds from two series were further characterized and shown to inhibit the nsP1 MTase activity. Conversely, these compounds barely inhibited a cellular MTase demonstrating their specificity towards nsP1. Analogues search and SAR were also initiated to identify the active pharmacophore features. Altogether the results show that this HT enzyme-based assay is a convenient way to select potent and specific hit compounds targeting the viral mRNA capping of Alphaviruses.

AB - Alphaviruses such as the Venezuelan equine encephalitis virus (VEEV) are important human emerging pathogens transmitted by mosquitoes. They possess a unique viral mRNA capping mechanism catalyzed by the viral non-structural protein nsP1, which is essential for virus replication. The alphaviruses capping starts by the methylation of a GTP molecule by the N7-guanine methyltransferase (MTase) activity; nsP1 then forms a covalent link with m 7 GMP releasing pyrophosphate (GT reaction) and the m 7 GMP is next transferred onto the 5′-diphosphate end of the viral mRNA to form a cap-0 structure. The cap-0 structure decreases the detection of foreign viral RNAs, prevents RNA degradation by cellular exonucleases, and promotes viral RNA translation into proteins. Additionally, reverse-genetic studies have demonstrated that viruses mutated in nsP1 catalytic residues are both impaired towards replication and attenuated. The nsP1 protein is thus considered an attractive antiviral target for drug discovery. We have previously demonstrated that the guanylylation of VEEV nsP1 can be monitored by Western blot analysis using an antibody recognizing the cap structure. In this study, we developed a high throughput ELISA screening assay to monitor the GT reaction through m 7 GMP-nsP1 adduct quantitation. This assay was validated using known nsP1 inhibitors before screening 1220 approved compounds. 18 compounds inhibiting the nsP1 guanylylation were identified, and their IC 50 determined. Compounds from two series were further characterized and shown to inhibit the nsP1 MTase activity. Conversely, these compounds barely inhibited a cellular MTase demonstrating their specificity towards nsP1. Analogues search and SAR were also initiated to identify the active pharmacophore features. Altogether the results show that this HT enzyme-based assay is a convenient way to select potent and specific hit compounds targeting the viral mRNA capping of Alphaviruses.

UR - https://www.scopus.com/pages/publications/85060441580

U2 - 10.1016/j.antiviral.2019.01.003

DO - 10.1016/j.antiviral.2019.01.003

M3 - Journal articles

C2 - 30639438

AN - SCOPUS:85060441580

SN - 0166-3542

VL - 163

SP - 59

EP - 69

JO - Antiviral Research

JF - Antiviral Research

ER -

Approved drugs screening against the nsP1 capping enzyme of Venezuelan equine encephalitis virus using an immuno-based assay

Abstract

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