期刊
CELL HOST & MICROBE
卷 18, 期 2, 页码 243-253出版社
CELL PRESS
DOI: 10.1016/j.chom.2015.06.019
关键词
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资金
- UC Berkeley Miller Institute
- NIH [R01CA136367, R01CA160556]
- Burroughs Wellcome Fund Investigator in the Pathogenesis of Infectious Disease Award
- W.M. Keck Foundation Distinguished Young Scientist Award
- Gordon and Betty Moore Foundation
Gamma-herpesviruses encode a cytoplasmic mRNA-targeting endonuclease, SOX, that cleaves most cellular mRNAs. Cleaved fragments are subsequently degraded by the cellular 5'-3' mRNA exonuclease Xrn1, thereby suppressing cellular gene expression and facilitating viral evasion of host defenses. We reveal that mammalian cells respond to this widespread cytoplasmic mRNA decay by altering RNA Polymerase II (RNAPII) transcription in the nucleus. Measuring RNAPII recruitment to promoters and nascent mRNA synthesis revealed that the majority of affected genes are transcriptionally repressed in SOX-expressing cells. The transcriptional feedback does not occur in response to the initial viral endonuclease-induced cleavage, but instead to degradation of the cleaved fragments by cellular exonucleases. In particular, Xrn1 catalytic activity is required for transcriptional repression. Notably, viral mRNA transcription escapes decay-induced repression, and this escape requires Xrn1. Collectively, these results indicate that mRNA decay rates impact transcription and that gamma-herpesviruses use this feedback mechanism to facilitate viral gene expression.
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