Cleavage of Dicer protein by I7 protease during vaccinia virus infection.

Dicer is the key component in the miRNA pathway. Degradation of Dicer protein is facilitated during vaccinia virus (VV) infection. A C-terminal cleaved product of Dicer protein was detected in the presence of MG132 during VV infection. Thus, it is possible that Dicer protein is cleaved by a viral pr...

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Main Authors: Jhih-Si Chen, Hui-Chun Li, Shu-I Lin, Chee-Hing Yang, Wan-Yu Chien, Ciao-Ling Syu, Shih-Yen Lo
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2015-01-01
Series:PLoS ONE
Online Access:http://europepmc.org/articles/PMC4376780?pdf=render
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spelling doaj-11f6f48b60b44137aab8631e34fc09242020-11-25T01:58:59ZengPublic Library of Science (PLoS)PLoS ONE1932-62032015-01-01103e012039010.1371/journal.pone.0120390Cleavage of Dicer protein by I7 protease during vaccinia virus infection.Jhih-Si ChenHui-Chun LiShu-I LinChee-Hing YangWan-Yu ChienCiao-Ling SyuShih-Yen LoDicer is the key component in the miRNA pathway. Degradation of Dicer protein is facilitated during vaccinia virus (VV) infection. A C-terminal cleaved product of Dicer protein was detected in the presence of MG132 during VV infection. Thus, it is possible that Dicer protein is cleaved by a viral protease followed by proteasome degradation of the cleaved product. There is a potential I7 protease cleavage site in the C-terminus of Dicer protein. Indeed, reduction of Dicer protein was detected when Dicer was co-expressed with I7 protease but not with an I7 protease mutant protein lack of the protease activity. Mutation of the potential I7 cleavage site in the C-terminus of Dicer protein resisted its degradation during VV infection. Furthermore, Dicer protein was reduced dramatically by recombinant VV vI7Li after the induction of I7 protease. If VV could facilitate the degradation of Dicer protein, the process of miRNA should be affected by VV infection. Indeed, accumulation of precursor miR122 was detected after VV infection or I7 protease expression. Reduction of miR122 would result in the suppression of HCV sub-genomic RNA replication, and, in turn, the amount of viral proteins. As expected, significant reduction of HCVNS5A protein was detected after VV infection and I7 protease expression. Therefore, our results suggest that VV could cleave Dicer protein through I7 protease to facilitate Dicer degradation, and in turn, suppress the processing of miRNAs. Effect of Dicer protein on VV replication was also studied. Exogenous expression of Dicer protein suppresses VV replication slightly while knockdown of Dicer protein does not affect VV replication significantly.http://europepmc.org/articles/PMC4376780?pdf=render
collection DOAJ
language English
format Article
sources DOAJ
author Jhih-Si Chen
Hui-Chun Li
Shu-I Lin
Chee-Hing Yang
Wan-Yu Chien
Ciao-Ling Syu
Shih-Yen Lo
spellingShingle Jhih-Si Chen
Hui-Chun Li
Shu-I Lin
Chee-Hing Yang
Wan-Yu Chien
Ciao-Ling Syu
Shih-Yen Lo
Cleavage of Dicer protein by I7 protease during vaccinia virus infection.
PLoS ONE
author_facet Jhih-Si Chen
Hui-Chun Li
Shu-I Lin
Chee-Hing Yang
Wan-Yu Chien
Ciao-Ling Syu
Shih-Yen Lo
author_sort Jhih-Si Chen
title Cleavage of Dicer protein by I7 protease during vaccinia virus infection.
title_short Cleavage of Dicer protein by I7 protease during vaccinia virus infection.
title_full Cleavage of Dicer protein by I7 protease during vaccinia virus infection.
title_fullStr Cleavage of Dicer protein by I7 protease during vaccinia virus infection.
title_full_unstemmed Cleavage of Dicer protein by I7 protease during vaccinia virus infection.
title_sort cleavage of dicer protein by i7 protease during vaccinia virus infection.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2015-01-01
description Dicer is the key component in the miRNA pathway. Degradation of Dicer protein is facilitated during vaccinia virus (VV) infection. A C-terminal cleaved product of Dicer protein was detected in the presence of MG132 during VV infection. Thus, it is possible that Dicer protein is cleaved by a viral protease followed by proteasome degradation of the cleaved product. There is a potential I7 protease cleavage site in the C-terminus of Dicer protein. Indeed, reduction of Dicer protein was detected when Dicer was co-expressed with I7 protease but not with an I7 protease mutant protein lack of the protease activity. Mutation of the potential I7 cleavage site in the C-terminus of Dicer protein resisted its degradation during VV infection. Furthermore, Dicer protein was reduced dramatically by recombinant VV vI7Li after the induction of I7 protease. If VV could facilitate the degradation of Dicer protein, the process of miRNA should be affected by VV infection. Indeed, accumulation of precursor miR122 was detected after VV infection or I7 protease expression. Reduction of miR122 would result in the suppression of HCV sub-genomic RNA replication, and, in turn, the amount of viral proteins. As expected, significant reduction of HCVNS5A protein was detected after VV infection and I7 protease expression. Therefore, our results suggest that VV could cleave Dicer protein through I7 protease to facilitate Dicer degradation, and in turn, suppress the processing of miRNAs. Effect of Dicer protein on VV replication was also studied. Exogenous expression of Dicer protein suppresses VV replication slightly while knockdown of Dicer protein does not affect VV replication significantly.
url http://europepmc.org/articles/PMC4376780?pdf=render
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