Protein Kinase C-Independent Activation of the Epstein-Barr Virus Lytic Cycle

Gradoville, Lyndle; Kwa, David; El-Guindy, Ayman; Miller, George

doi:10.1128/jvi.76.11.5612-5626.2002

Cited by 80 publications

(89 citation statements)

References 58 publications

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“…For herpesviruses, the ability to induce replication depends on not only the type of CMR but also the type of cell line being induced (Gradoville et al, 2002). The lack of persistently infected cell lines does not help attempts to isolate CFPHV, so we tried to get around this problem by using early subculture cells known to contain CFPHV pol DNA.…”

Section: Discussionmentioning

confidence: 99%

In vitro biology of fibropapilloma-associated turtle herpesvirus and host cells in Hawaiian green turtles (Chelonia mydas)

Work

Dagenais

Balazs

et al. 2009

Journal of General Virology

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Fibropapillomatosis (FP) of green turtles has a global distribution and causes debilitating tumours of the skin and internal organs in several species of marine turtles. FP is associated with a presently non-cultivable alphaherpesvirus Chelonid fibropapilloma-associated herpesvirus (CFPHV). Our aims were to employ quantitative PCR targeted to pol DNA of CFPHV to determine (i) if DNA sequesters by tumour size and/or cell type, (ii) whether subculturing of cells is a viable strategy for isolating CFPHV and (iii) whether CFPHV can be induced to a lytic growth cycle in vitro using chemical modulators of replication (CMRs), temperature variation or co-cultivation. Additional objectives included determining whether non-tumour and tumour cells behave differently in vitro and confirming the phenotype of cultured cells using cell-type-specific antigens. CFPHV pol DNA was preferentially concentrated in dermal fibroblasts of skin tumours and the amount of viral DNA per cell was independent of tumour size. Copy number of CFPHV pol DNA per cell rapidly decreased with cell doubling of tumour-derived fibroblasts in culture. Attempts to induce viral replication in known CFPHV-DNA-positive cells using temperature or CMR failed. No significant differences were seen in in vitro morphology or growth characteristics of fibroblasts from tumour cells and paired normal skin, nor from CFPHV pol-DNA-positive intestinal tumour cells. Tumour cells were confirmed as fibroblasts or keratinocytes by positive staining with antivimentin and anti-pancytokeratin antibodies, respectively. CFPHV continues to be refractory to in vitro cultivation.

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Section: Discussionmentioning

confidence: 99%

In vitro biology of fibropapilloma-associated turtle herpesvirus and host cells in Hawaiian green turtles (Chelonia mydas)

Work

Dagenais

Balazs

et al. 2009

Journal of General Virology

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“…It has been reported that latently infected LCL can be driven to enter into the lytic phase of the EBV life cycle by exposure to PMA, a protein kinase C agonist, and sodium butyrate (NaB), a histone deacetylase inhibitor (Bhaduri-McIntosh & Miller, 2006;Gradoville et al, 2002), so protein lysates were prepared from LCL that were either treated with PMA þ NaB or left untreated. In three out of four animals tested, a higher frequency of LCV-specific cells was detected when lysate from PMA/NaBtreated LCL was used as the source of LCV antigen (Figure 2a).…”

Section: Optimization Of the Lcv Antigen Used In The Ifn-c Elispot Assaymentioning

confidence: 99%

“…The presence of LCV genome and protein expression of LCV latent and lytic phase proteins were confirmed (refer to supplemental data section for additional details). Lysates were prepared from non-treated LCL or LCL treated with 20 ng phorbol-12-myristate 13-acetate (PMA)/ml (Sigma, St. Louis, MO) þ 3 mM sodium butyrate (NaB) (Sigma) for 72 h to enhance LCV gene expression (Gradoville et al, 2002). Lot-specific titers for use in the IFN-g ELISPOT assay were determined from dose-response curves; both LCV seronegative and seropositive PBMC were routinely tested to ensure specificity of responses.…”

Section: Antigensmentioning

confidence: 99%

Measuring T-cell responses against LCV and CMV in cynomolgus macaques using ELISPOT: Potential application to non-clinical testing of immunomodulatory therapeutics

Kamperschroer

O’Donnell

Schneider

et al. 2013

Journal of Immunotoxicology

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A number of immunomodulatory therapeutics increase the risk of disease associated with latent herpesviruses such as cytomegalovirus (CMV) and Epstein-Barr virus (EBV), a member of the lymphocryptovirus (LCV) family that infects humans. The diseases associated with loss of immunity to these viruses can have major impacts on patients as well as on the commercial viability of the immunomodulatory therapeutics. In an effort to develop non-clinical methods for measuring effects on anti-viral immunity, we have developed an interferon (IFN)-g enzymelinked immunosorbent spot (ELISPOT) assay to quantify the number of CMV or LCV-reactive Tcells in peripheral blood of cynomolgus macaques. After optimization of various parameters, the IFN-g ELISPOT assay was characterized for specificity, intra-assay, monkey-to-monkey, and longitudinal variability and sensitivity to immunosuppression. The results show that nearly all animals have detectable responses against both CMV and LCV and responses were derived from T-cells specific to the virus of interest. Analyses of variability show assay reproducibility ( 23% CV), and that variability over time in anti-viral responses in individual animals (larger for LCV than for CMV) was $2-fold in most animals over a 3-month time period, which is predicted to allow for detection of drug-induced changes when using group sizes typical of non-clinical studies. In addition, the IFN-g ELISPOT assay was capable of detecting decreases in the numbers of CMV and LCV reactive T-cells induced by immunosuppressive drugs in vitro. This assay may allow for non-clinical assessment of the effects of immunomodulatory therapeutics on anti-viral T-cell immunity in monkeys, and may help determine if therapeutics increase the risk of reactivating latent viral infections.

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“…The inducing effect of phorbol esters is mediated through protein kinase C (PKC) (Davies et al, 1991), and also primarily requires the ZI and ZII binding motifs in the BZLF1 promoter , although the intermediary factors are not well defined. However, PKC activation is not required for induction of lytic EBV by certain stimuli (Gradoville et al, 2002). Activation of the BRLF1 (Rp) promoter requires EGR-1 and Sp1 binding sites (Zalani et al, 1992(Zalani et al, , 1995.…”

Section: Induction Of Lytic Ebv Infectionmentioning

confidence: 99%