Genome-Wide CRISPR Screen Identifies RACK1 as a Critical Host Factor for Flavivirus Replication

被引:42
作者
Shue, Byron [1 ]
Chiramel, Abhilash, I [2 ]
Cerikan, Berati [3 ]
Thu-Hien To [4 ]
Froelich, Sonja [1 ]
Pederson, Stephen M. [4 ]
Kirby, Emily N. [1 ]
Eyre, Nicholas S. [1 ,5 ]
Bartenschlager, Ralf F. W. [3 ]
Best, Sonja M. [2 ]
Beard, Michael R. [1 ]
机构
[1] Univ Adelaide, Res Ctr Infect Dis, Dept Mol & Biomed Sci, Adelaide, SA, Australia
[2] NIH, Rocky Mt Labs, Hamilton, MT USA
[3] Heidelberg Univ, Dept Infect Dis, Mol Virol, D-69120 Heidelberg, Germany
[4] Univ Adelaide, Bioinformat Hub, Adelaide, SA, Australia
[5] Flinders Univ S Australia, Coll Med & Publ Hlth, Bedford Pk, SA 5042, Australia
来源
JOURNAL OF VIROLOGY | 2021年 / 95卷 / 24期
基金
英国医学研究理事会;
关键词
ZIKV; crispr; flavivirus; host factor; organelle; screen; viral replication; C VIRUS NS5A; ZIKA VIRUS; DENGUE VIRUS; WEST-NILE; PROTEIN; TRANSLATION; BIOGENESIS; ACTIVATION; KNOCKOUT; VIRULENT;
D O I
10.1128/JVI.00596-21
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
Cellular factors have important roles in all facets of the flavivirus replication cycle. Deciphering viral-host protein interactions is essential for understanding the flavivirus life cycle as well as development of effective antiviral strategies. To uncover novel host factors that are co-opted by multiple flaviviruses, a CRISPR/Cas9 genome wide knockout (KO) screen was employed to identify genes required for replication of Zika virus (ZIKV). Receptor for Activated Protein C Kinase 1 (RACK1) was identified as a novel host factor required for ZIKV replication, which was confirmed via complementary experiments. Depletion of RACK1 via siRNA demonstrated that RACK1 is important for replication of a wide range of mosquito- and tick-borne flaviviruses, including West Nile Virus (WNV), Dengue Virus (DENY), Powassan Virus (POWV) and Langat Virus (LGTV) as well as the coronavirus SARS-CoV-2, but not for YFV, EBOV, VSV or HSV. Notably, flavivirus replication was only abrogated when RACK1 expression was dampened prior to infection. Utilising a non-replicative flavivirus model, we show altered morphology of viral replication factories and reduced formation of vesicle packets (VPs) in cells lacking RACK1 expression. In addition, RACK1 interacted with NS1 protein from multiple flaviviruses; a key protein for replication complex formation. Overall, these findings reveal RACK1's crucial role to the biogenesis of pan-flavivirus replication organelles. IMPORTANCE Cellular factors are critical in all facets of viral lifecycles, where overlapping interactions between the virus and host can be exploited as possible avenues for the development of antiviral therapeutics. Using a genome-wide CRISPR knockout screening approach to identify novel cellular factors important for flavivirus replication we identified RACK1 as a pro-viral host factor for both mosquito- and tick-borne flaviviruses in addition to SARS-CoV-2. Using an innovative flavivirus protein expression system, we demonstrate for the first time the impact of the loss of RACK1 on the formation of viral replication factories known as 'vesicle packets' (VPs). In addition, we show that RACK1 can interact with numerous flavivirus NS1 proteins as a potential mechanism by which VP formation can be induced by the former.
引用
收藏
页数:18
相关论文
共 55 条
[1]   RACK1, A multifaceted scaffolding protein: Structure and function [J].
Adams, David R. ;
Ron, Dorit ;
Kiely, Patrick A. .
CELL COMMUNICATION AND SIGNALING, 2011, 9
[2]   Shaping the flavivirus replication complex: It is curvaceous! [J].
Aktepe, Turgut E. ;
Mackenzie, Jason M. .
CELLULAR MICROBIOLOGY, 2018, 20 (08)
[3]   The Host Protein Reticulon 3.1A Is Utilized by Flaviviruses to Facilitate Membrane Remodelling [J].
Aktepe, Turgut E. ;
Liebscher, Susann ;
Prier, Julia E. ;
Simmons, Cameron P. ;
Mackenzie, Jason M. .
CELL REPORTS, 2017, 21 (06) :1639-1654
[4]   Mutational analysis of hepatitis C virus nonstructural protein 5A: Potential role of differential phosphorylation in RNA replication and identification of a genetically flexible domain [J].
Appel, N ;
Pietschmann, T ;
Bartenschlager, R .
JOURNAL OF VIROLOGY, 2005, 79 (05) :3187-3194
[5]   Comparison of the Live Attenuated Yellow Fever Vaccine 17D-204 Strain to Its Virulent Parental Strain Asibi by Deep Sequencing [J].
Beck, Andrew ;
Tesh, Robert B. ;
Wood, Thomas G. ;
Widen, Steven G. ;
Ryman, Kate D. ;
Barrett, Alan D. T. .
JOURNAL OF INFECTIOUS DISEASES, 2014, 209 (03) :334-344
[6]   RACK1 is indispensable for porcine reproductive and respiratory syndrome virus replication and NF-κB activation in Marc-145 cells [J].
Bi, Junlong ;
Zhao, Qian ;
Zhu, Lingyun ;
Li, Xidan ;
Yang, Guishu ;
Liu, Jianping ;
Yin, Gefen .
SCIENTIFIC REPORTS, 2018, 8
[7]   A Non-Replicative Role of the 3′ Terminal Sequence of the Dengue Virus Genome in Membranous Replication Organelle Formation [J].
Cerikan, Berati ;
Goellner, Sarah ;
Neufeldt, Christopher John ;
Haselmann, Uta ;
Mulder, Klaas ;
Chatel-Chaix, Laurent ;
Cortese, Mirko ;
Bartenschlager, Ralf .
CELL REPORTS, 2020, 32 (01)
[8]   Dengue Virus- and Hepatitis C Virus- Induced Replication and Assembly Compartments: the Enemy Inside-Caught in the Web [J].
Chatel-Chaix, Laurent ;
Bartenschlager, Ralf .
JOURNAL OF VIROLOGY, 2014, 88 (11) :5907-5911
[9]   TRIM5α Restricts Flavivirus Replication by Targeting the Viral Protease for Proteasomal Degradation [J].
Chiramel, Abhilash, I ;
Meyerson, Nicholas R. ;
McNally, Kristin L. ;
Broeckel, Rebecca M. ;
Montoya, Vanessa R. ;
Mendez-Solis, Omayra ;
Robertson, Shelly J. ;
Sturdevant, Gail L. ;
Lubick, Kirk J. ;
Nair, Vinod ;
Youseff, Brian H. ;
Ireland, Robin M. ;
Bosio, Catharine M. ;
Kim, Kyusik ;
Luban, Jeremy ;
Hirsch, Vanessa M. ;
Taylor, R. Travis ;
Bouamr, Fadila ;
Sawyer, Sara L. ;
Best, Sonja M. .
CELL REPORTS, 2019, 27 (11) :3269-+
[10]   Role of autophagy in Zika virus infection and pathogenesis [J].
Chiramel, Abhilash I. ;
Best, Sonja M. .
VIRUS RESEARCH, 2018, 254 :34-40
123456