Distribution and Phosphorylation of the Basic Protein P6.9 of Autographa californica Nucleopolyhedrovirus

Liu, Xiaoxiao; Zhao, Haizhou; Fang, Zhang; Yuan, Meijin; Yang, Kai; Pang, Yi

doi:10.1128/jvi.00438-12

Cited by 19 publications

(32 citation statements)

References 34 publications

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“…However, the capsid structures resulting from loss of the aforementioned genes were located not only in the RZ but also in the VS (interspace of the electron-dense mats) (16,(18)(19)(20)22), whereas in vAc54KO-transfected cells, no capsid structures were observed in the VS (Fig. 2B).…”

Section: Resultsmentioning

confidence: 94%

“…In addition, abnormal electron-dense bodies were found in the VS, and empty capsid structures were found in the RZ in cells transfected with vAc54KO, indicating that ablation of ac54 disrupted the normal assembly of nucleocapsids. In addition to ac54, some other AcMNPV genes (i.e., 38K, ac53, ac83, pk-1, and p6.9) have also been implicated in nucleocapsid assembly, and their individual deletion results in the cessation of assembly and the appearance of empty capsid structures in both the RZ and VS (16)(17)(18)(19)(20)22). However, in the present study, neither capsid structures nor VP39 was observed inside the VS in Sf9 cells transfected with vAc54KO, implying a special role of VP1054 in the baculovirus life cycle besides nucleocapsid assembly.…”

Section: Discussionmentioning

confidence: 99%

“…Autographa californica multiple nucleopolyhedrovirus (AcMNPV) is the most intensively studied baculovirus. In addition to the major capsid protein VP39 (11,12), AcMNPV nucleocapsids contain several minor components (6,13), such as the following: P6.9, a protamine-like protein that is responsible for the condensation of viral DNA to form the nucleocapsid core (14)(15)(16); PK-1, a virus-encoded protein kinase that is required for the hyperphosphorylation of P6.9, which facilitates the release of viral DNA from the nucleocapsid (17); and 38K, Ac53, VP91 (encoded by ac83), and VLF-1, which are also classified as minor capsid proteins although their exact functions are poorly understood (18)(19)(20)(21). Single deletion of the genes encoding each of the six minor capsid proteins mentioned above results in the failure of nucleocapsid assembly and the distribution of abnormally long electron-lucent tubular structures at the electrondense edges of the stroma, indicating that the packaging of DNA and nucleoproteins into capsids is interrupted (16,(18)(19)(20)(21)(22).…”

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confidence: 99%

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The Autographa californica Multiple Nucleopolyhedrovirus ac54 Gene Is Crucial for Localization of the Major Capsid Protein VP39 at the Site of Nucleocapsid Assembly

Guan

Zhong

et al. 2016

J Virol

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Baculovirus DNAs are synthesized and inserted into preformed capsids to form nucleocapsids at a site in the infected cell nucleus, termed the virogenic stroma. Nucleocapsid assembly of Autographa californica multiple nucleopolyhedrovirus (AcMNPV) requires the major capsid protein VP39 and nine minor capsid proteins, including VP1054. However, how VP1054 participates in nucleocapsid assembly remains elusive. In this study, the VP1054-encoding gene (ac54) was deleted to generate the ac54-knockout AcMNPV (vAc54KO). In vAc54KO-transfected cells, nucleocapsid assembly was disrupted, leading to the formation of abnormally elongated capsid structures. Interestingly, unlike cells transfected with AcMNPV mutants lacking other minor capsid proteins, in which capsid structures were distributed within the virogenic stroma, ac54 ablation resulted in a distinctive location of capsid structures and VP39 at the periphery of the nucleus. The altered distribution pattern of capsid structures was also observed in cells transfected with AcMNPV lacking BV/ODV-C42 or in cytochalasin D-treated AcMNPV-infected cells. BV/ODV-C42, along with PP78/83, has been shown to promote nuclear filamentous actin (F-actin) formation, which is another requisite for nucleocapsid assembly. Immunofluorescence using phalloidin indicated that the formation and distribution of nuclear F-actin were not affected by ac54 deletion. However, immunoelectron microscopy revealed that BV/ODV-C42, PP78/83, and 38K failed to integrate into capsid structures in the absence of VP1054, and immunoprecipitation further demonstrated that in transient expression assays, VP1054 interacted with BV/ODV-C42 and VP80 but not VP39. Our findings suggest that VP1054 plays an important role in the transport of capsid proteins to the nucleocapsid assembly site prior to the process of nucleocapsid assembly. IMPORTANCEBaculoviruses are large DNA viruses whose replication occurs within the host nucleus. The localization of capsids into the capsid assembly site requires virus-induced nuclear F-actin; the inhibition of nuclear F-actin formation results in the retention of capsid structures at the periphery of the nucleus. In this paper, we note that the minor capsid protein VP1054 is essential for the localization of capsid structures, the major capsid protein VP39, and the minor capsid protein 38K into the capsid assembly site. Moreover, VP1054 is crucial for correct targeting of the nuclear F-actin factors BV/ODV-C42 and PP78/83 for capsid maturation. However, the formation and distribution of nuclear F-actin are not affected by the lack of VP1054. We further reveal that VP1054 interacts with BV/ODV-C42 and a capsid transport-related protein, VP80. Taken together, our findings suggest that VP1054 plays a unique role in the pathway(s) for transport of capsid proteins. The family Baculoviridae includes a diverse group of insect-specific viruses that contain circular double-stranded DNA within a rod-shaped protein capsid enclosed by a lipid envelope (1, 2). Two forms of virions (bu...

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Section: Resultsmentioning

confidence: 94%

Section: Discussionmentioning

confidence: 99%

mentioning

confidence: 99%

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The Autographa californica Multiple Nucleopolyhedrovirus ac54 Gene Is Crucial for Localization of the Major Capsid Protein VP39 at the Site of Nucleocapsid Assembly

Guan

Zhong

et al. 2016

J Virol

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“…Furthermore, many different dephosphorylated forms of P6.9, as well as phosphorylated P6.9, were present in association with ODVs, although only dephosphorylated P6.9 was associated with BVs . P6.9 was also detected in the BV proteomes of HearNPV and AcMNPV, but not in the BV proteome of AgMNPV, which might be a result of P6.9 cleavage (Braconi et al, 2014;Liu et al, 2012). The biological significance of the cleavage of P6.9 remains unclear.…”

Section: Proteins Shared By Seven Identified Baculovirusesmentioning

confidence: 99%

Proteomic analysis of the occlusion-derived virus of Clostera anachoreta granulovirus

Zhang

Liang

et al. 2015

Journal of General Virology

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To date, proteomic studies have been performed on occlusion-derived viruses (ODVs) from five members of the family Baculoviridae, genus Alphabaculovirus, but only a single member of the genus Betabaculovirus (Pieris rapae granulovirus). In this study, LC-MS/MS was used to analyse the ODV proteins of Clostera anachoreta granulovirus (ClanGV), another member of the genus Betabaculovirus. The results indicated that 73 proteins, including the products of 27 baculovirus core genes, were present in ClanGV ODVs. This is the largest number of ODV proteins identified in baculoviruses to date. To the best of our knowledge, 24 of these proteins were newly identified as ODV-associated proteins. Twelve of the proteins were shared by all seven of the other baculoviruses that have been analysed by proteomic techniques, including P49, PIF-2, ODV-EC43, P74, P6.9, P33, VP39, ODV-EC27, VP91, GP41, VLF-1 and VP1054. ClanGV shared between 20 and 36 ODV proteins with each of the other six baculoviruses that have been analysed by proteomics. Ten proteins were identified only as ODV components of ClanGV and PrGV: Clan22, Clan27, Clan69, Clan83, Clan84, Clan90, Clan116, Clan94, FGF-3 and ME53, the first seven of which were encoded by betabaculovirus-specific genes. These findings may provide novel insights into baculovirus structure as well as reveal similarities and differences between alphabaculoviruses and betabaculoviruses.

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“…To explore the mechanism by which ac132 influences assembly and envelopment of nucleocapsids, experiments were performed to detect interaction between AC132 and other viral proteins. The candidate proteins selected for examination included the major capsid protein VP39 (39), the viral genome-binding protein P6.9 (41,42), BV and ODV envelope proteins E25 (40) and E18 (43), VS-associated proteins IE1 (44) and PP31 (45), and BV/ODV-C42, involved in virus-induced nuclear actin polymerization (46). The extracts of Sf9 cells infected by AcMNPV were immunoprecipitated with AC132-specific antibodies.…”

Section: Ac132mentioning

confidence: 99%

Autographa californica Multiple Nucleopolyhedrovirus orf132 Encodes a Nucleocapsid-Associated Protein Required for Budded-Virus and Multiply Enveloped Occlusion-Derived Virus Production

Yang

Wang

Yue

et al. 2014

J Virol

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Autographa californica multiple nucleopolyhedrovirus orf132 (named ac132) has homologs in all genome-sequenced group I nucleopolyhedroviruses. Its role in the viral replication cycle is unknown. In this study, ac132 was shown to express a protein of around 28 kDa, which was determined to be associated with the nucleocapsids of both occlusion-derived virus and budded virus. Confocal microscopy showed that AC132 protein appeared in central region of the nucleus as early as 12 h postinfection with the virus. It formed a ring zone at the periphery of the nucleus by 24 h postinfection. To investigate its role in virus replication, ac132 was deleted from the viral genome by using a bacmid system. In the Sf9 cell culture transfected by the ac132 knockout bacmid, infection was restricted to single cells, and the titer of infectious budded virus was reduced to an undetectable level. However, viral DNA replication and the expression of late genes vp39 and odv-e25 and a reporter gene under the control of the very late gene p10 promoter were unaffected. Electron microscopy showed that nucleocapsids, virions, and occlusion bodies were synthesized in the cells transfected by an ac132 knockout bacmid, but the formation of the virogenic stroma and occlusion bodies was delayed, the numbers of enveloped nucleocapsids were reduced, and the occlusion bodies contained mainly singly enveloped nucleocapsids. AC132 was found to interact with envelope protein ODV-E18 and the viral DNA-binding protein P6.9. The data from this study suggest that ac132 possibly plays an important role in the assembly and envelopment of nucleocapsids. IMPORTANCETo our knowledge, this is the first report on a functional analysis of ac132. The data presented here demonstrate that ac132 is required for production of the budded virus and multiply enveloped occlusion-derived virus of Autographa californica multiple nucleopolyhedrovirus. This article reveals unique phenotypic changes induced by ac132 deletion on the virus and multiple new findings on ac132.

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Distribution and Phosphorylation of the Basic Protein P6.9 of Autographa californica Nucleopolyhedrovirus

Cited by 19 publications

References 34 publications

The Autographa californica Multiple Nucleopolyhedrovirus ac54 Gene Is Crucial for Localization of the Major Capsid Protein VP39 at the Site of Nucleocapsid Assembly

The Autographa californica Multiple Nucleopolyhedrovirus ac54 Gene Is Crucial for Localization of the Major Capsid Protein VP39 at the Site of Nucleocapsid Assembly

Proteomic analysis of the occlusion-derived virus of Clostera anachoreta granulovirus

Autographa californica Multiple Nucleopolyhedrovirus orf132 Encodes a Nucleocapsid-Associated Protein Required for Budded-Virus and Multiply Enveloped Occlusion-Derived Virus Production

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