Influenza virus genome C4 promoter/origin attenuates its transcription and replication activity by the low polymerase recognition activity

Hongbing Jiang; Shijian Zhang; Qiang Wang; Jinlan Wang; Liqing Geng; Tetsuya Toyoda

doi:10.1016/j.virol.2010.09.022

Influenza virus genome C4 promoter/origin attenuates its transcription and replication activity by the low polymerase recognition activity

Hongbing Jiang, Shijian Zhang, Qiang Wang, Jinlan Wang, Liqing Geng, Tetsuya Toyoda

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

10 Scopus citations

Abstract

A natural variation is observed at position 4 of the 3' -end of influenza A virus genomes, where U (U4) or C (C4) is present. The replicon activity of C4 was 28% of U4. We compared the transcription and replication activity of U4 [v84(U4)], C4 [v84(C4)] and the complimentary RNA (c84) using the purified influenza virus RNA polymerase in vitro. ApG-primed replication activities of v84(C4) and c84 were 23.8% and 7.8% of v84(U4). Globin mRNA-primed transcription activities of v84(C4) and c84 were 36.9% and 6.81% of v84(U4). De novo replication activities of v84(C4) and c84 were 21.3 and 10.2% of v84(U4). This difference came from their polymerase binding activity. When all the eight genome segments of WSN strain were changed to U4, the virus titer was 760 times higher than the wild type. However, its pathogenicity in mice was lower than the wild type.

Original language	English (US)
Pages (from-to)	190-196
Number of pages	7
Journal	Virology
Volume	408
Issue number	2
DOIs	https://doi.org/10.1016/j.virol.2010.09.022
State	Published - Dec 20 2010

Keywords

Influenza virus
Interferon
NS1
RNA polymerase
Replication origin
Transcription promoter

ASJC Scopus subject areas

Virology

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10.1016/j.virol.2010.09.022

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@article{95ebfeb261634565985fd44471ef4802,

title = "Influenza virus genome C4 promoter/origin attenuates its transcription and replication activity by the low polymerase recognition activity",

abstract = "A natural variation is observed at position 4 of the 3' -end of influenza A virus genomes, where U (U4) or C (C4) is present. The replicon activity of C4 was 28% of U4. We compared the transcription and replication activity of U4 [v84(U4)], C4 [v84(C4)] and the complimentary RNA (c84) using the purified influenza virus RNA polymerase in vitro. ApG-primed replication activities of v84(C4) and c84 were 23.8% and 7.8% of v84(U4). Globin mRNA-primed transcription activities of v84(C4) and c84 were 36.9% and 6.81% of v84(U4). De novo replication activities of v84(C4) and c84 were 21.3 and 10.2% of v84(U4). This difference came from their polymerase binding activity. When all the eight genome segments of WSN strain were changed to U4, the virus titer was 760 times higher than the wild type. However, its pathogenicity in mice was lower than the wild type.",

keywords = "Influenza virus, Interferon, NS1, RNA polymerase, Replication origin, Transcription promoter",

author = "Hongbing Jiang and Shijian Zhang and Qiang Wang and Jinlan Wang and Liqing Geng and Tetsuya Toyoda",

note = "Funding Information: We thank Drs. Y. Kawaoka, G. Hobom, T. Fujita and M. Stinski for the 12-plasmid influenza reconstitution systems, pHH21, p-125Luc and pCMV1, respectively. This work was supported by Grants-in-aid from the Chinese Academy of Sciences ( 0514P51131 ), National Science Foundation of China ( 30670090 , 30970153 ), Li Ka Shing Foundation ( 0682P11131 ), RESPARI ( 0581P14131 ), and FLUINNATE ( SP5B-CT-2006-044161 ).",

year = "2010",

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doi = "10.1016/j.virol.2010.09.022",

language = "English (US)",

volume = "408",

pages = "190--196",

journal = "Virology",

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T1 - Influenza virus genome C4 promoter/origin attenuates its transcription and replication activity by the low polymerase recognition activity

AU - Jiang, Hongbing

AU - Zhang, Shijian

AU - Wang, Qiang

AU - Wang, Jinlan

AU - Geng, Liqing

AU - Toyoda, Tetsuya

N1 - Funding Information: We thank Drs. Y. Kawaoka, G. Hobom, T. Fujita and M. Stinski for the 12-plasmid influenza reconstitution systems, pHH21, p-125Luc and pCMV1, respectively. This work was supported by Grants-in-aid from the Chinese Academy of Sciences ( 0514P51131 ), National Science Foundation of China ( 30670090 , 30970153 ), Li Ka Shing Foundation ( 0682P11131 ), RESPARI ( 0581P14131 ), and FLUINNATE ( SP5B-CT-2006-044161 ).

PY - 2010/12/20

Y1 - 2010/12/20

N2 - A natural variation is observed at position 4 of the 3' -end of influenza A virus genomes, where U (U4) or C (C4) is present. The replicon activity of C4 was 28% of U4. We compared the transcription and replication activity of U4 [v84(U4)], C4 [v84(C4)] and the complimentary RNA (c84) using the purified influenza virus RNA polymerase in vitro. ApG-primed replication activities of v84(C4) and c84 were 23.8% and 7.8% of v84(U4). Globin mRNA-primed transcription activities of v84(C4) and c84 were 36.9% and 6.81% of v84(U4). De novo replication activities of v84(C4) and c84 were 21.3 and 10.2% of v84(U4). This difference came from their polymerase binding activity. When all the eight genome segments of WSN strain were changed to U4, the virus titer was 760 times higher than the wild type. However, its pathogenicity in mice was lower than the wild type.

AB - A natural variation is observed at position 4 of the 3' -end of influenza A virus genomes, where U (U4) or C (C4) is present. The replicon activity of C4 was 28% of U4. We compared the transcription and replication activity of U4 [v84(U4)], C4 [v84(C4)] and the complimentary RNA (c84) using the purified influenza virus RNA polymerase in vitro. ApG-primed replication activities of v84(C4) and c84 were 23.8% and 7.8% of v84(U4). Globin mRNA-primed transcription activities of v84(C4) and c84 were 36.9% and 6.81% of v84(U4). De novo replication activities of v84(C4) and c84 were 21.3 and 10.2% of v84(U4). This difference came from their polymerase binding activity. When all the eight genome segments of WSN strain were changed to U4, the virus titer was 760 times higher than the wild type. However, its pathogenicity in mice was lower than the wild type.

KW - Influenza virus

KW - Interferon

KW - NS1

KW - RNA polymerase

KW - Replication origin

KW - Transcription promoter

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C2 - 20956010

AN - SCOPUS:78149406275

SN - 0042-6822

VL - 408

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EP - 196

JO - Virology

JF - Virology

IS - 2

ER -

Influenza virus genome C4 promoter/origin attenuates its transcription and replication activity by the low polymerase recognition activity

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