Myristoylation of the RING Finger Z Protein Is Essential for Arenavirus Budding

Perez, Mar; Greenwald, Dori L.; Torre, Juan Carlos de la

doi:10.1128/jvi.78.20.11443-11448.2004

Cited by 119 publications

(143 citation statements)

References 37 publications

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“…Rib inhibits arenavirus replication via mechanisms that have not been entirely elucidated but most likely involve the targeting of different steps of virus RNA synthesis (21). However, 2-OHM inhibits myristoylation of Z, which is required for arenavirus budding (22). Based on their mechanisms of action, we predicted that Rib would similarly inhibit production of virus progeny upon infection at low or high moi, whereas the inhibitory effect of 2-OHM would be expected to be more pronounced in infections initiated at low moi involving multiple rounds of cell infection required for virus propagation within the cell population.…”

Section: Assessment Of R3lcmv As a Novel Tool To Identify Antiarenaviralmentioning

confidence: 99%

Generation of recombinant lymphocytic choriomeningitis viruses with trisegmented genomes stably expressing two additional genes of interest

Emonet

Garidou

McGavern

et al. 2009

Proc. Natl. Acad. Sci. U.S.A.

121

216

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Several arenaviruses cause hemorrhagic fever disease in humans for which no licensed vaccines are available and current therapeutic intervention is limited to the off-label use of the wide-spectrum antiviral ribavirin. However, the prototypic arenavirus lymphocytic choriomeningitis virus (LCMV) has proven to be a Rosetta stone for the investigation of virus-host interactions. Arenaviruses have a bisegmented negative-strand RNA genome. The S segment encodes for the virus nucleoprotein and glycoprotein, whereas the L segment encodes for the virus polymerase (L) and Z protein. The ability to generate recombinant LCMV (rLCMV) expressing additional foreign genes of interest would open novel avenues for the study of virushost interactions and the development of novel vaccine strategies and high-throughput screens to identify antiarenaviral molecules. To this end, we have developed a trisegmented (1L ؉ 2S) rLCMV-based approach (r3LCMV). Each of the two S segments in r3LCMV was altered to replace one of the viral genes by a gene of interest. All r3LCMVs examined expressing different reported genes were stable both genetically and phenotypically and exhibited wild-type growth properties in cultured cells. Reporter gene expression in r3LCMV-infected cells provided an accurate surrogate of levels of virus multiplication. Notably, some r3LCMVs displayed highly attenuated virulence in mice but induced protective immunity against a subsequent lethal challenge with wild-type LCMV, supporting the potential development of r3LCMV-based vaccines.antiviral screen ͉ reverse genetic ͉ viral attenuation A renaviruses merit significant interest both as tractable experimental model systems to study acute and persistent viral infections and as clinically important human pathogens (1-3). Thus, the prototypic arenavirus lymphocytic choriomeningitis virus (LCMV) has proven to be a superb workhorse in the field of virology and immunology (1). However, several arenaviruses cause hemorrhagic fever (HF) disease in humans, associated with high morbidity and mortality (2, 3). The Old World arenavirus Lassa virus (LASV) poses the highest public health concern among HF arenaviruses. LASV is estimated to infect several hundred thousand individuals yearly in its endemic region of West Africa, resulting in a high number of Lassa fever disease cases (2). Likewise, several New World arenaviruses, chiefly Junin virus, cause viral HF disease (3). Moreover, evidence indicates that the worldwide distributed LCMV is a neglected human pathogen of clinical significance (4) and poses a special threat to immunocompromised individuals (5, 6).Public health concerns posed by human pathogenic arenaviruses are aggravated by the lack of licensed vaccines and current therapy being limited to the use of the nucleoside analog ribavirin (Rib) that can cause significant side effects and requires an early and i.v. administration for optimal efficacy (3). Therefore, it is important to develop novel effective antiarenaviral drugs and vaccines, tasks that would be facilitated ...

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Section: Assessment Of R3lcmv As a Novel Tool To Identify Antiarenaviralmentioning

confidence: 99%

Generation of recombinant lymphocytic choriomeningitis viruses with trisegmented genomes stably expressing two additional genes of interest

Emonet

Garidou

McGavern

et al. 2009

Proc. Natl. Acad. Sci. U.S.A.

121

216

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“…We recently demonstrated that the PPXY late domain in LCMV Z is not absolutely required for the production of infectious LCMV virions (Ziegler et al, 2016). Provided that the only other motif in Z with a known role in budding activity is the myristoylation site at the glycine at position 2 (Figs 1c and 2d) (Perez et al, 2004;Strecker et al, 2006), our finding here expands the functional repertoire of motifs in LCMV Z that regulate the efficiency of infectious virus release. Further, we have built upon our previous findings regarding the PPXY late domain (Ziegler et al, 2016) by showing that S41 also serves as a key regulator of DI particle formation.…”

mentioning

confidence: 53%

“…To determine whether the reduction in infectious titre of the phosphomimetic S41D virus was due to decreased virus budding and release, we employed a Z VLP release assay as previously described (Ziegler et al, 2016). As a control, we also included the LCMV Z G2A mutant, which exhibits a pronounced defect in VLP formation due to its inability to be myristoylated at this glycine residue (Perez et al, 2004;Strecker et al, 2006). This experiment demonstrated that the budding efficiency of the phosphomimetic Z-S41D was reduced~60 %, while the budding activity of the nonphosphorylatable S41A was not different from WT (Fig.…”

mentioning

confidence: 99%

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A novel phosphoserine motif in the LCMV matrix protein Z regulates the release of infectious virus and defective interfering particles

Ziegler

Eisenhauer

Bruce

et al. 2016

Journal of General Virology

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We report that the lymphocytic choriomeningitis virus (LCMV) matrix protein, which drives viral budding, is phosphorylated at serine 41 (S41). A recombinant (r)LCMV bearing a phosphomimetic mutation (S41D) was impaired in infectious and defective interfering (DI) particle release, while a non-phosphorylatable mutant (S41A) was not. The S41D mutant was disproportionately impaired in its ability to release DI particles relative to infectious particles. Thus, DI particle production by LCMV may be dynamically regulated via phosphorylation of S41.

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“…It is the main driving force of virion budding (Salvato et al, 1992;Strecker et al, 2003). It contains a conserved RING-fi nger domain fl anked by an Nterminal hydrophobic domain with myristoylation and phosphorylation site (Perez et al, 2004). Th e C-terminal portion of ZP contains proline-rich motifs that have been identifi ed as late motifs in matrix proteins (Eichler et al, 2004;Freed, 2002).…”

Section: Z Proteinmentioning

confidence: 99%

Lymphocytic choriomeningitis virus: ways to establish and maintain non-cytolytic persistent infection

Labudová¹,

Pastorek²,

Pastoreková³

2016

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Summary. -Lymphocytic choriomeningitis virus (LCMV) is a prototype virus of the Arenaviridae family that is attracting considerable attention both as an important experimental model system to study acute and persistent viral infections, and as a neglected human pathogen of clinical signifi cance. Notably, LCMV is capable of persisting in an infected host, and escaping the immune system. Here we describe the strategies used by the virus to establish and maintain long-term infection in vitro and/or persistent infection in vivo. We discuss how the viral components (RNA, nucleoprotein, glycoprotein, Z protein) manipulate the host cell machinery to facilitate survival and spread of the virus without disturbing the basal cellular processes. Deep understanding of these strategies is inevitable for the development of approaches towards restricting the virus spread and/or preventing its harmful reactivation. Th is review summarizes the current status in this area and presents ideas emerging from existing data.Keywords: lymphocytic choriomeningitis virus; arenaviruses; persistent infection E-mail: virulama@savba.sk; phone: +421-2-59302439. Abbreviations: ATF6 = activating transcription factor 6; DC = dendritic cells; DG = dystroglycan; ECM = extracellular matrix; eIF-4E/G = eukaryotic translation initiation factor 4E or 4G; eIF-4G = eukaryotic translation initiation factor 4G; GAPDH = glyceraldehyd-3-phosphate dehydrogenase; GP1,2 = glycoprotein 1, 2; GPC = glycoprotein precursor; IRE1 = inositol-requiring protein 1; IRF-3 = IFN regulatory factor 3; PERK = PKR-like ER kinase; PML = promyelocytic leukemia; UPR = unfolded protein response; ZP = Z protein

show abstract

Myristoylation of the RING Finger Z Protein Is Essential for Arenavirus Budding

Cited by 119 publications

References 37 publications

Generation of recombinant lymphocytic choriomeningitis viruses with trisegmented genomes stably expressing two additional genes of interest

Generation of recombinant lymphocytic choriomeningitis viruses with trisegmented genomes stably expressing two additional genes of interest

A novel phosphoserine motif in the LCMV matrix protein Z regulates the release of infectious virus and defective interfering particles

Lymphocytic choriomeningitis virus: ways to establish and maintain non-cytolytic persistent infection

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