Duck Plague Virus pUL48 Protein Activates the Immediate-Early Gene to Initiate the Transcription of the Virus Gene

Duck plague caused by the duck plague virus (DPV) is an infectious disease that seriously harms the waterfowl breeding industry. The VP16 protein of α herpesvirus can bind to specific cis-acting elements upstream of the promoter of the immediate-early (IE, α) gene to promote the transcription of the...

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Autores principales: Zhou, Tong, Fan, Dengjian, Wang, Mingshu, Cheng, Anchun, Wu, Ying, Yang, Qiao, Tian, Bin, Jia, Renyong, Ou, Xumin, Mao, Sai, Sun, Di, Zhang, Shaqiu, Zhu, Dekang, Chen, Shun, Liu, Mafeng, Zhao, Xin-Xin, Huang, Juan, Gao, Qun, Yu, Yanling, Zhang, Ling
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Frontiers Media S.A. 2021
Materias:
Microbiology
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8733724/
https://www.ncbi.nlm.nih.gov/pubmed/35003026
http://dx.doi.org/10.3389/fmicb.2021.795730
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author Zhou, Tong
Fan, Dengjian
Wang, Mingshu
Cheng, Anchun
Wu, Ying
Yang, Qiao
Tian, Bin
Jia, Renyong
Ou, Xumin
Mao, Sai
Sun, Di
Zhang, Shaqiu
Zhu, Dekang
Chen, Shun
Liu, Mafeng
Zhao, Xin-Xin
Huang, Juan
Gao, Qun
Yu, Yanling
Zhang, Ling
author_facet Zhou, Tong
Fan, Dengjian
Wang, Mingshu
Cheng, Anchun
Wu, Ying
Yang, Qiao
Tian, Bin
Jia, Renyong
Ou, Xumin
Mao, Sai
Sun, Di
Zhang, Shaqiu
Zhu, Dekang
Chen, Shun
Liu, Mafeng
Zhao, Xin-Xin
Huang, Juan
Gao, Qun
Yu, Yanling
Zhang, Ling
author_sort Zhou, Tong
collection PubMed
description Duck plague caused by the duck plague virus (DPV) is an infectious disease that seriously harms the waterfowl breeding industry. The VP16 protein of α herpesvirus can bind to specific cis-acting elements upstream of the promoter of the immediate-early (IE, α) gene to promote the transcription of the IE gene, so it is also called the trans-inducer of IE gene (α-TIF). However, no studies on DPV α-TIF have been reported. This study investigated the DPV pUL48, a homolog of HSV-1 VP16, transcriptional activation region, target sequence, and viral protein affecting its transcriptional activation using a dual-luciferase reporter gene detection system, and pUL48 was identified as the α-TIF of DPV. (1) The regulation of pUL48 on DPV different gene promoters showed that pUL48 could activate all the promoters of IE genes (ICP4, ICP22, and ICP27) but not the promoters of early and late genes. (2) The activity of pUL48 to ICP4 and ICP22 promoters with different upstream lengths showed that pUL48 activated ICP4 and ICP22 promoters by acting on TAATGA (T) TAT element upstream of ICP4 promoter and TAATTATAT element upstream of ICP22 promoter, respectively. (3) Transcriptional activation of IE gene by truncated proteins of different lengths at the N-terminal of pUL48 was detected. The results showed that the transcriptional activation domain of pUL48 was amino acids 1–60 at the N-terminal, and amino acids 1–20 was its core region. In addition, it was found that pUL14, pUL46, and pUL47 significantly promoted the transcriptional activation of pUL48. The effects of loss of pUL47 and its nuclear localization signal on the nuclear entry and transcriptional activation function of pUL48 were further examined. The results showed that pUL47 could promote the nuclear entry of pUL48 through its nuclear localization signal at positions 40–50 and 768–777 amino acids, thus, enhancing the transcriptional activation function of pUL48 and synergistic promotion of viral gene transcription.
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spelling pubmed-87337242022-01-07 Duck Plague Virus pUL48 Protein Activates the Immediate-Early Gene to Initiate the Transcription of the Virus Gene Zhou, Tong Fan, Dengjian Wang, Mingshu Cheng, Anchun Wu, Ying Yang, Qiao Tian, Bin Jia, Renyong Ou, Xumin Mao, Sai Sun, Di Zhang, Shaqiu Zhu, Dekang Chen, Shun Liu, Mafeng Zhao, Xin-Xin Huang, Juan Gao, Qun Yu, Yanling Zhang, Ling Front Microbiol Microbiology Duck plague caused by the duck plague virus (DPV) is an infectious disease that seriously harms the waterfowl breeding industry. The VP16 protein of α herpesvirus can bind to specific cis-acting elements upstream of the promoter of the immediate-early (IE, α) gene to promote the transcription of the IE gene, so it is also called the trans-inducer of IE gene (α-TIF). However, no studies on DPV α-TIF have been reported. This study investigated the DPV pUL48, a homolog of HSV-1 VP16, transcriptional activation region, target sequence, and viral protein affecting its transcriptional activation using a dual-luciferase reporter gene detection system, and pUL48 was identified as the α-TIF of DPV. (1) The regulation of pUL48 on DPV different gene promoters showed that pUL48 could activate all the promoters of IE genes (ICP4, ICP22, and ICP27) but not the promoters of early and late genes. (2) The activity of pUL48 to ICP4 and ICP22 promoters with different upstream lengths showed that pUL48 activated ICP4 and ICP22 promoters by acting on TAATGA (T) TAT element upstream of ICP4 promoter and TAATTATAT element upstream of ICP22 promoter, respectively. (3) Transcriptional activation of IE gene by truncated proteins of different lengths at the N-terminal of pUL48 was detected. The results showed that the transcriptional activation domain of pUL48 was amino acids 1–60 at the N-terminal, and amino acids 1–20 was its core region. In addition, it was found that pUL14, pUL46, and pUL47 significantly promoted the transcriptional activation of pUL48. The effects of loss of pUL47 and its nuclear localization signal on the nuclear entry and transcriptional activation function of pUL48 were further examined. The results showed that pUL47 could promote the nuclear entry of pUL48 through its nuclear localization signal at positions 40–50 and 768–777 amino acids, thus, enhancing the transcriptional activation function of pUL48 and synergistic promotion of viral gene transcription. Frontiers Media S.A. 2021-12-23 /pmc/articles/PMC8733724/ /pubmed/35003026 http://dx.doi.org/10.3389/fmicb.2021.795730 Text en Copyright © 2021 Zhou, Fan, Wang, Cheng, Wu, Yang, Tian, Jia, Ou, Mao, Sun, Zhang, Zhu, Chen, Liu, Zhao, Huang, Gao, Yu and Zhang. https://creativecommons.org/licenses/by/4.0/This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) and the copyright owner(s) are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
spellingShingle Microbiology
Zhou, Tong
Fan, Dengjian
Wang, Mingshu
Cheng, Anchun
Wu, Ying
Yang, Qiao
Tian, Bin
Jia, Renyong
Ou, Xumin
Mao, Sai
Sun, Di
Zhang, Shaqiu
Zhu, Dekang
Chen, Shun
Liu, Mafeng
Zhao, Xin-Xin
Huang, Juan
Gao, Qun
Yu, Yanling
Zhang, Ling
Duck Plague Virus pUL48 Protein Activates the Immediate-Early Gene to Initiate the Transcription of the Virus Gene
title Duck Plague Virus pUL48 Protein Activates the Immediate-Early Gene to Initiate the Transcription of the Virus Gene
title_full Duck Plague Virus pUL48 Protein Activates the Immediate-Early Gene to Initiate the Transcription of the Virus Gene
title_fullStr Duck Plague Virus pUL48 Protein Activates the Immediate-Early Gene to Initiate the Transcription of the Virus Gene
title_full_unstemmed Duck Plague Virus pUL48 Protein Activates the Immediate-Early Gene to Initiate the Transcription of the Virus Gene
title_short Duck Plague Virus pUL48 Protein Activates the Immediate-Early Gene to Initiate the Transcription of the Virus Gene
title_sort duck plague virus pul48 protein activates the immediate-early gene to initiate the transcription of the virus gene
topic Microbiology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8733724/
https://www.ncbi.nlm.nih.gov/pubmed/35003026
http://dx.doi.org/10.3389/fmicb.2021.795730
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