Epstein-Barr Virus Down-Regulates Tumor Suppressor Expression
Many oncogenic viruses exhibit cellular transforming properties, often involving oncogenes activation and tumor suppressor genes inactivation. The DOK1 gene is a newly identified tumor suppressor gene with altered expression via hypermethylation of its promoter in a variety of human cancers, including head and neck, lung, gastric and others. In addition, a correlation has been reported between DOK1 aberrant hypermethylation and the presence of oncogenic viruses such as hepatitis B virus (HBV) in hepatocellular carcinoma (HCC) and Epstein-Barr virus (EBV) in Burkitt's lymphoma-derived cell lines. Here we demonstrate for the first time that EBV is directly involved in the inhibition of DOK1 expression in B-cells. We show that EBV leads to epigenetic repression of DOK1 through increased DNA methylation of its promoter and H3K27 tri-methylation. The LMP1 oncoprotein plays a key role in the repression of DOK1 expression. It promotes the formation and the recruitment to the DOK1 promoter of transcriptionally inhibitory complexes composed of E2F1/pRB/DNMT1 and of EZH2 which is part of the polycomb repressive complex 2. Interestingly, one or more additional EBV protein(s) cooperate(s) with LMP1 in inducing massive DNA methylation at the DOK1 promoter, leading to the loss of E2F1 complexes recruitment and even stronger repression of DOK1 expression.
Published in the journal:
. PLoS Pathog 10(5): e32767. doi:10.1371/journal.ppat.1004125
Category:
Research Article
doi:
https://doi.org/10.1371/journal.ppat.1004125
Summary
Many oncogenic viruses exhibit cellular transforming properties, often involving oncogenes activation and tumor suppressor genes inactivation. The DOK1 gene is a newly identified tumor suppressor gene with altered expression via hypermethylation of its promoter in a variety of human cancers, including head and neck, lung, gastric and others. In addition, a correlation has been reported between DOK1 aberrant hypermethylation and the presence of oncogenic viruses such as hepatitis B virus (HBV) in hepatocellular carcinoma (HCC) and Epstein-Barr virus (EBV) in Burkitt's lymphoma-derived cell lines. Here we demonstrate for the first time that EBV is directly involved in the inhibition of DOK1 expression in B-cells. We show that EBV leads to epigenetic repression of DOK1 through increased DNA methylation of its promoter and H3K27 tri-methylation. The LMP1 oncoprotein plays a key role in the repression of DOK1 expression. It promotes the formation and the recruitment to the DOK1 promoter of transcriptionally inhibitory complexes composed of E2F1/pRB/DNMT1 and of EZH2 which is part of the polycomb repressive complex 2. Interestingly, one or more additional EBV protein(s) cooperate(s) with LMP1 in inducing massive DNA methylation at the DOK1 promoter, leading to the loss of E2F1 complexes recruitment and even stronger repression of DOK1 expression.
Introduction
Cellular transformation induced by oncogenic viruses often involves the activation of growth-promoting signaling pathways and the inactivation of tumor suppressor genes. The downstream of tyrosine kinase 1gene (DOK1) has emerged as a newly identified tumor suppressor gene that encodes a multi-domain adapter protein and acts as a negative regulator of signaling pathways involved in several cellular functions. DOK1 inhibits cell proliferation, down regulates MAP kinase activity, and has an opposing role in leukemogenesis and promotes cell spreading, motility, and apoptosis [1], [2]. Functional studies showed that mice lacking the DOK1 and/or DOK2 genes have a high susceptibility to the development of lung adenocarcinomas [3] and exhibit significant defects in their immune responses and immune cell development, often developing myelo-proliferative and autoimmune diseases, e.g. lupus-like renal disease [4], [5]. The DOK1 gene locus is located in the human chromosome 2p13 region, which is frequently rearranged in a number of human tumors [6]. Oncogenic tyrosine kinases such as p210BCR-ABL, the causative mutation in chronic myelogenous leukemia (CML), and Src target DOK1 for ubiquitin-mediated proteasomal degradation [7], therefore promoting cell proliferation. We have reported a frameshift mutation of the DOK1 gene in chronic lymphoid leukemia (CLL) resulting in the expression of truncated DOK1 that is exclusively localized in the nucleus and loses its tumor suppressive activities, in contrast with the cytoplasmic wild type protein [8]. We also showed that DOK1 gene expression is repressed in a large proportion of head and neck cancer (HNC), lung cancer and Burkitt's lymphoma [9], as a result of aberrant hypermethylation of its promoter region. The inactivation of DOK1 through promoter methylation also occurred in liver and gastric cancers [10], [11]. Thus, DOK1 emerged as a tumor suppressor frequently altered in a variety of human cancers, making it a potential marker and therapeutic target in cancer control.
Epstein-Barr virus (EBV) is a γ-herpes-virus that is widespread in 90% of human populations. In the majority of individuals, EBV persists as a permanent, asymptomatic infection of the lymphocytes B-lymphocyte pool [12]. EBV occasionally causes infectious mononucleosis in adolescents [13] and is considered a human carcinogenic infectious agent. Indeed, EBV is associated with the development of different types of B-cell lymphoma such as Burkitt's lymphoma (BL), Hodgkin disease, lympho-proliferative disorders in immuno-deficient individuals, and nasopharyngeal carcinoma [14], [15], [16]. EBV is also associated with gastric cancer [17]. The oncogenic potential of EBV has been further demonstrated by its ability to immortalize efficiently the primary human B-cells in vitro in lymphoblastoid cell lines (LCLs) [18]. LCLs carry the EBV genome in an extra-chromosomal episome state and express nine latent viral proteins: three trans-membrane proteins (LMP1, LMP2A and 2B) and six nuclear antigens (EBNAs 1, 2, 3A, 3B, 3C and LP), along with other non-translated RNA products [12]. These viral products enhance the proliferation of quiescent B-cells and maintain the viral genome in its episomal form. However, only EBNA1, 2, 3A, 3C, LP, and LMP1 are essential for the transformation of primary B-cells into LCLs [19]. The latent membrane protein 1 (LMP1) is crucial for EBV-induced B-cell immortalization. It is the only EBV latent protein that displays transforming properties in vitro [20].
LMP1 protein is thought to alter cell growth transformation by mimicking the activated forms of tumor necrosis factor receptor (TNFR), CD40 and CD30 receptors [21], [22], [23]. Through its long C-terminal cytosolic domain, LMP1 has the ability to induce several signaling pathways, including the MAP kinase (both ERK/MAPK and p38/MAPK), nuclear factor kappa B (NF-κB) and c-Jun N-terminal kinase (JNK) [24], [25], [26], [27]. The alteration of these signaling pathways by LMP1 is essential for the oncogenicity of EBV.
The presence of the EBV genome in several lymphomas, and its ability to induce B-cell immortalization, and alter host-cell expression profiles and epigenome (i.e. DNA methylation patterns) strongly support an etiological role for EBV in these cancers. We recently reported that the expression of DOK1 gene is repressed through DNA hypermethylation in BL cell lines, it became of interest to investigate the possible role of EBV in the inhibition of DOK1 expression in infected B-cells. To date, very little is known about the regulation of DOK1 expression by oncogenic viruses.
In the present study, we demonstrate a strong association between EBV infection and DOK1 gene silencing via hypermethylation of its promoter in EBV-infected cell lines. We show that EBV infection in B-cells leads to epigenetic repression and CpG methylation of the DOK1 gene and that LMP1 expression inhibits DOK1 promoter activity via the recruitment of inhibitory complexes including E2F1, pRB, DNMT1 and EZH2.
Results
EBV infection of primary human B-cells in vitro leads to down-regulation of DOK1 expression
Based on our previous results that showed the down-regulation of DOK1 expression in BL cell-lines [9], we evaluate whether this event was linked to infection with EBV, a key risk factor for this malignancy. Primary human B-cells, isolated from different healthy donors, were infected in independent experiments with recombinant EBV virus expressing the green fluorescent protein (GFP-EBV). The infection efficiency was evaluated by flow cytometry to monitor GFP expression (data not shown). The expression of EBV genes EBNA1 and LMP1, as well as DOK1 was determined by real-time PCR and western blot at different time points post-infection (Figure 1A and B). EBV infection resulted in a strong reduction of DOK1 mRNA and protein levels, which was evident at 16 hours post-infection (Figure 1A). Similarly, DOK1 mRNA and protein levels were strongly down-regulated by EBV in three cancers B-cell lines (RPMI, BJAB and Louckes) infected by EBV, as well as in EBV-immortalized lymphoblastoid cells lines (LCLs) (Figure 1C and D). Together, these findings highlight a role for EBV in down-regulating DOK1 gene expression.
LMP1 plays a key role in the inhibition of DOK1 expression
The EBV oncoprotein LMP1 is essential for EBV-induced B-cell immortalization by altering cellular gene expression via the activation of several signaling pathways [28]. To determine whether LMP1 can affect the expression of DOK1, we infected the RPMI cells with wild-type GFP-EBV or GFP-EBV lacking the LMP1 gene (EBVΔLMP1). The infection efficiency was monitored using flow cytometry for GFP expression (Figure 2A). In contrast to wild-type GFP-EBV, EBVΔLMP1 infection in primary B cells and in RPMI cells did not significantly decrease DOK1 mRNA or protein levels (Figure 2B and C). Re-expression of LMP1 in EBVΔLMP1 RPMI cells by retroviral transduction restored the ability of EBV to down-regulate DOK1 expression, while transduction of the same cells with empty retrovirus (pLXSN) did not affect DOK1 mRNA or protein levels (Figure 2D and E), highlighting the key role of LMP1 in this event. Accordingly, expression of LMP1 alone in RPMI cells was sufficient to reduce DOK1 mRNA and protein expression (Figure 2D and E), whereas expression of other viral proteins, such as EBNA1, 2, 3A, 3B, and 3C, did not lead to down-regulation of DOK1 protein levels (supplementary Figure S1A–C) In addition, transient transfection of RPMI with increasing concentrations of LMP1 expressing vector resulted in the decrease of DOK1 expression is a dose dependent manner (Figure 2F and G). Together, these data underline the key role of LMP1 in EBV-mediated DOK1 down-regulation in infected B-cells.
LMP1 down-regulates DOK1 expression by altering the composition of the E2F transcription complex
We recently showed that the E2F1 transcription factor has a key role in activation of DOK1 transcription [29]. The 500 nucleotide upstream of the start site of the DOK1 promoter contains three E2F1 responsive elements (RE) which appear to have a role in transcription activation; in particular the one at position −498/−486 (ERE1) [29]. Transient transfection experiments showed that LMP1 was able to efficiently inhibit the activity of −500/+33 DOK1 promoter cloned in front of the luciferase reporter gene (Figure 3A). The addition of upstream regions (−1000/−500 or −2000/−500) did not modify the pattern of LMP1 inhibition (Figure 3A). In addition, LMP1 was not able to further decrease the activity of DOK1 promoter harboring point mutations in ERE1 (Figure 3A). Together, these results suggest that LMP1 may exert its inhibitory activity targeting the regulatory complexes able to bind ERE1 within the −500/+33 region of the DOK1 promoter. Chromatin immuno-precipitation (ChIP) experiments using an anti-E2F1 antibody showed that infection with wild-type GFP-EBV significantly decreases the recruitment of E2F1 to ERE1 in RPMI and two independent LCLs (Figure 3B), while EBVΔLMP1 did not have any impact on this event in RPMI (Figure 3B). Interestingly, LMP1 alone did not prevent the recruitment of E2F1 to the DOK1 promoter in RPMI cells (Figure 3B), although it is able to efficiently down-regulate DOK1 expression (Figures 2D, 2E, and 3A).
We next analyzed the chromatin organization within the DOK1 promoter in the same cells by monitoring the tri-methylation of histone H3 at lysine 4 (H3K4me3) or at lysine 27 (H3K27me3) which are events associated with transcriptionally active or inactive chromatin, respectively. According to their ability to repress DOK1 expression, wild-type GFP-EBV or LMP1 alone induced an increase of H3K27me3 and a decrease of H3K4me3 within the DOK1 promoter compared with mock cells (Figure 3C). However, LMP1 was less efficient than the entire virus in promoting these epigenetic changes (Figure 3C). In summary, although LMP1 alone is not able to prevent the recruitment of E2F1 to the DOK1 promoter, it is capable of inducing epigenetic changes and inhibition of DOK1 transcription.
Based on these findings, we hypothesized that LMP1 mediates DOK1 down-regulation by altering the composition of the E2F1 complex. To explore this possibility, we performed oligo pull-down experiments using biotinylated DNA probes which contain a region of the DOK1 promoter encompassing the wild-type or mutated ERE1. Biotinylated DNA probes were incubated with protein extracts from RPMI cells transduced with empty retrovirus or with retrovirus expressing LMP1. In both extracts and as expected, E2F1 was found associated with the DNA, while only in the presence of LMP1 were three additional cellular proteins, which are usually part of negative regulatory complexes of transcription found associated with the DOK1 promoter fragment: (i) the E2F1 inhibitor retinoblastoma (pRB), (ii) the DNA methyl-transferase DNMT1 and (iii) the polycomb-group (PcG) 2 member EZH2 (Figure 3D). Deletion of ERE1 prevented the association of E2F1 in both cellular extracts. In addition, in LMP1-containing extracts, mutation of ERE1 also significantly decreased the pRB and DNMT1 protein levels precipitated with DNA (Figure 3D), suggesting that both proteins are recruited in the same complex as E2F1. With regard to EZH2, its binding to the DOK1 promoter was less affected by the ERE1 mutation, indicating that it is recruited by a different complex. Although LMP1 is able to activate the NF-κB pathway, no binding of the p65 transcription factor was found in both cellular extracts (Figure 3D). ChIP Re-ChIP experiments in mock and LMP1-expressing cells confirmed the data obtained in the pull-down assay. Indeed, Re-ChIP showed that a significant proportion of E2F1 complexes recruited to the DOK1 promoter contains pRB and DNMT1 proteins (80% and 40% respectively), but not EZH2 (Figure 3E), which appears to be associated with an independent complex.
Finally, the events occurring at DOK1 promoter were determined at early stages post-infection with EBV. We observed a significant enrichment of pRB, DNMT1 and EZH2 recruitment to DOK1 promoter in primary naive B cells infected with recombinant GFP-EBV virus for 48 hours. Consequently, an increase of H3K27 trimethylation (∼5 folds) and CpG methylation (∼10%) was detected (Supplementary Figure S3). Thus, early stage of EBV infection mimics the scenario observed in LMP1-expressing cells.
In summary, these data show that LMP1 initiates the repression of DOK1 expression by inducing the formation of transcriptional inhibitory complexes.
LMP1-mediated NF-κB activation is required for DOK1 down-regulation
LMP1 has the ability to activate different signaling pathways, such as NF-κB, MAPK p38, JNK, and MAPK/ERK [28]. To explore the potential role of these pathways in DOK1 down-regulation, RPMI cells infected with recombinant GFP-EBV were treated with different chemical inhibitors specific for these signaling pathways. No change was observed in mock or GFP-EBV cells treated with the chemical inhibitors of the MAPK p38, JNK, and MAPK/ERK pathways (SB203580, S600125 and PD98059, respectively) (data not shown). However, DOK1 mRNA and protein levels were found to be considerably increased in GFP-EBV-infected cells treated with a specific inhibitor of NF-κB (Bay11), but not in mock cells (Figure 4A and B). Similarly, Bay11 treatment of LMP1-expressing cells increased the DOK1 mRNA and protein levels (Figure 4A and B). To further demonstrate the role of NF-κB signaling in EBV-mediated DOK1 down-regulation, we inhibited the NF-κB canonical pathway by expressing a non-degradable deletion mutant of IκBα (Δ-IκBα) that lacks the first 36 amino acids at the N-terminus containing the IKK-phosphorylated amino acid. Similarly to Bay 11, Δ-IκBα expression in GFP-EBV RPMI cells led to an increase of transcript and protein levels of DOK1 (Figure 4C and D). Accordingly, transient transfection experiments using a plasmid containing the DOK1 promoter cloned upstream of the luciferase gene showed that Δ-IκBα antagonized LMP1 in inhibiting the DOK1 promoter (Supplementary Figure S2).
The LMP1 protein has two important C-terminal cytosolic domains named C-terminal activation region 1 (CTAR-1) (residues 194–232) and 2 (CTAR-2) (residues 351–386). Both the CTAR1 and CTAR2 domains have the ability to activate the NF-κB pathway through their interactions with tumor necrosis factor receptor (TNFR)-associated factors (TRAFs) [30], and TNFR-associated death domain protein (TRADD) [31], respectively. In particular, the CTAR2 domain is required for the activation of the canonical NF-κB pathway, while the CTAR1 domain is critical for the stimulation of the non-canonical NF-κB pathway [32]. The LMP1 mutants AxAxA (mutated CTAR1), 378 stop (deleted in CTAR2) and AxAxA/378 stop (mutated CTAR1 and deleted CTAR2) were expressed in RPMI cells. Both LMP1 378 stop and AxAxA/378 stop mutants failed to down-regulate the DOK1 gene, but not the LMP1 AxAxA mutant, which still retained its ability to suppress DOK1 expression at similar levels of wild-type LMP1 (Figure 4E and F). Therefore, LMP1 down-regulates DOK1 expression through its CTAR2 domain. In addition, we investigated whether the LMP1-mediated NF-κB activation plays a role in the formation of inhibitory complexes and their recruitment to the DOK1 promoter. LMP1-expressing RPMI cells were cultured in the presence of NF-κB inhibitor Bay11. No significant change in pRB and DMNT1 intracellular levels was observed, whereas EZH2 levels were slightly decreased (Figure 4H). However, oligo pull-down experiments clearly showed that inhibition of the NF-κB signaling affected the binding efficiency of pRB and DNMT1 to DOK1 promoter, while E2F1 and EZH2 continued to be associated with the DNA (Figure 4H). ChIP assay confirmed that inhibition of NF-κB significantly decreased the recruitment of pRB and DNMT1 to the DOK1 promoter (Figure 4G). Together, the data show that activation of the canonical NF-κB pathway by LMP1 is an important event for the down-regulation of DOK1 expression.
DOK1 gene silencing through DNA methylation is associated with EBV infection in B-cells
In our previous study [9], we reported that DOK1 expression is repressed in 64% of Burkitt's lymphoma cell lines through DNA hypermethylation of its promoter. These findings prompted us to assess whether hypermethylation of the DOK1 promoter could be ascribed to the presence of EBV. Using pyrosequencing and real-time PCR, respectively, DOK1 methylation and expression levels were measured in our experimental model. EBV infection of RPMI cells led to hypermethylation of DOK1 promoter (Figure 5A). This phenomenon was even more evident in LCLs (Figure 5A). EBVΔLMP1 was unable to promote DOK1 promoter methylation, further underlining the importance of the viral oncoprotein in this event. However, in agreement with the fact that LMP1 alone is unable to displace E2F1 from the DOK1 promoter, low DNA methylation was detected in RPMI cells expressing LMP1 alone (Figure 5A). In addition, no further methylation was observed in RPMI cells co-expressing LMP1 with other EBV proteins, i.e. EBNA3A, 3B, or 3C (data not shown), suggesting that a more complex pattern of viral gene expression is required to induce hypermethylation of DOK1 promoter. Treatments with the methyl-transferase inhibitor 5-Aza-2′-deoxycytidine (5-Aza) significantly affected DOK1 promoter methylation in LCLs and RPMI cells infected with EBV (Figure 5A). As expected, 5-Aza treatment rescued the recruitment of E2F1 to the DOK1 promoter in GFP-EBV infected cells, while no change was observed in LMP1-expressing cells (Figure 5B). However, an increase of DOK1 mRNA and protein levels was observed upon exposure to 5-Aza in GFP-EBV-infected cells (RPMI or LCLs) as well as in LMP1-expressing RPMI cells (Figure 5C and D). This event correlates with the decrease of H3K27me3 and the increase of H3K4me3 levels (Figure 5E).
Together, these data show that EBV induces hypermethylation of the DOK1 promoter. Although expression of LMP1 alone marginally promotes DNA methylation, deletion of its gene in the EBV genome prevents the occurrence of this event. Thus, LMP1 appears to be essential, but not sufficient for hypermethylation of the DOK1 promoter.
Re-expression of DOK1 in LCLs decreased cellular proliferation and induced apoptosis
To understand the biological significance of EBV-induced DOK1-down-regulation, we re-expressed DOK1 in LCLs. We observed that ectopic DOK1 levels decreased LCL proliferation in a dose-dependent manner (Figure 6A). Consistently with these observations, DOK1 induced a significance decrease of cell populations in G0/G1 and G2/M phases (Figure 6B). In addition, high levels of DOK1 led to a significant increase of subG0 population and AnnexinV-positive cells (Figure 6B and C).Together, these data demonstrate the role of DOK1 in inhibiting cell proliferation induced by EBV and promoting both cell growth arrest and apoptosis.
Discussion
Several studies have demonstrated that the loss of DOK1 function is a key event in human carcinogenesis [1], [3], [4], [9], [33]. Indeed several mechanisms of DOK1 inactivation have been characterized so far DOK1 expression was found to be silenced by hypermethylation of its promoter in a variety of human cancers, including, head and neck, lung, gastric and liver cancer as well as in Burkitt's lymphoma-derived cell lines [9], [10], [11]. In addition, DOK1 was found to be mutated in chronic lymphocytic leukemia (CLL) [8]. At the protein level, DOK1 is targeted for proteasome degradation triggered by oncoprotein kinases (OTKs) such as p210bcr-abl and oncogenic forms of Src [7].
A recent study has provided evidence that DOK1 inactivation also occurs in virus-induced cancers [10]. Indeed, a correlation between DOK1 aberrant hypermethylation and the presence of hepatitis B virus (HBV) has been reported in hepatocellular carcinoma (HCC) [10]. Similarly, the expression of DOK1 mRNA was found to be down-regulated in cell lines derived from Burkitt's lymphoma [34], a pathological condition associated with EBV infection. However, these initial findings do not provide evidence about whether the down-regulation of DOK1 expression is directly induced by the viral proteins or is a consequence of the chromosomal alterations occurring during the carcinogenic processes. In this study, we demonstrate for the first time that EBV is directly involved in the inhibition of DOK1 expression. Our data show that the EBV LMP1 oncoprotein plays a key role in this event. Indeed, an EBV mutant lacking the entire LMP1 gene was unable to inhibit DOK1 transcription, while re-expression of LMP1 in cells infected with the EBVΔLMP1 mutant fully restored the ability of EBV to decrease DOK1 mRNA and protein levels. Expression of LMP1 alone in human cancer B-cells was sufficient to efficiently inhibit DOK1 transcription by promoting the formation of a transcriptional repressor complex containing E2F1, pRB, and the DNA methyl-transferase DNMT1. In addition, deletion of the E2F1-binding element (ERE1) strongly affected the binding of three cellular proteins to the DOK1 promoter, and a Re-ChIP assay confirmed that E2F1 is the carrier of pRB and DNMT1. We also observed that LMP1 promotes the recruitment of the histone-lysine N-methyl-transferase EZH2 independently of E2F1, leading to an increase in the level of H3K27me3. In agreement with the recruitment of the two epigenetic enzymes, an increase in H3K27me3 and DNA methylation levels was detected at the DOK1 promoter.
It has previously been shown that LMP1 is able to increase the expression and activity of DNA methyl-transferases (DNMT 1, 3a, and 3b), which could explain the increase of the DOK1 promoter methylation. Interestingly, DNA methylation was strongly enhanced in B-cells infected by the entire virus compared with cells expressing only LMP1. Thus, it is likely that additional viral products may cooperate with LMP1 in promoting DOK1 silencing via DNA methylation. No down-regulation of DOK1 was observed when EBNA1, 2, 3A, 3B, and 3C are expressed in RPMI cells. In addition, none of these viral proteins further stimulate DNA methylation at DOK1 promoter when co-expressed with LMP1 (data not shown). Thus, a more complex pattern of viral gene expression may be involved in the hyper-methylation of DOK1 promoter. Most importantly, we show that in EBV-infected B-cells the DNA methylation extends over a large region of the DOK1 promoter including ERE1 that loses the ability to recruit the active form of E2F1. Inhibition of DNA methylation significantly increases DOK1 transcription in LMP1-expressing cells as well as EBV-infected cells.
In summary, based on our findings, a two-step model can be proposed for EBV in the inhibition of DOK1 expression (Figure 7). In the first step, LMP1 favors the formation and recruitment of transcriptional repressor complexes containing E2F1/pRB/DNMT1 and EZH2. These complexes induce epigenetic changes in the DOK1 promoter region, leading to its inhibition. In the second step, LMP1 in collaboration with other EBV proteins leads to further increase of DNA methylation which in turn results in a loss of all transcriptional regulatory complexes and a strong repression of the DOK1 promoter. These data corroborate our previous studies that highlighted the key role of E2F1 and DNA methylation in the regulation of DOK1 expression [29]. Our data also show that the LMP1-induced DOK1 down-regulation is linked to activation of the NF-κB canonical pathway. Indeed, NF-κB activation by LMP1 plays a role in the formation and recruitment of inhibitory complex E2F1/pRB/DNMT1 to the DOK1 promoter. Although we did not observe any recruitment of p65 to the DOK1 promoter, neither by DNA-pull-down assay nor by chromatin immuno-precipitation (data not shown), we cannot exclude the involvement of other NF-κB transcription factors.
Until now, several studies reported that DNA methylation patterns were higher in EBV positive tumors compared to the EBV-negative ones and that EBV infection was clearly demonstrated to induce specific methylation epigenotypes that lead to silencing of multiple tumor suppressor genes such as BIM, p16INK4A, p14ARF, p73, E-cadherin and PTEN in EBV–associated nasopharyngeal and gastric cancers [17], [35], [36], [37], [38]. While these events are believed to be caused by elevated levels of DNMTs induced by LMP1 and 2, the mechanisms establishing the methylation patterns themselves are unknown. As DNA methyl-transferases have little specificity in vitro, we propose the notion that LMP1 triggers DOK1 gene repression through the recruitment of DNMT1 to its promoter in a specific manner via E2F1-binding to its response element, and this event might be an early step for EBV-induced DNA methylation. As some of the genes listed above are targets of E2F1 [39], [40], it will be interesting to see whether their methylation patterns are also specific to the recruitment of the inhibitory complex E2F1/pRB/DNMT1. Moreover, EBV appears to have an initiator role of epigenetic alterations and therefore inducing oncogenesis, however, the latency expression patterns of EBV genes differ in different cancers, which make unclear the contribution of the virus to some types. One explanation would be that EBV-induced epigenetic changes, such as EBV-mediated DNA methylation of DOK1 promoter, are stable events and could also persist even after the changes in EBV latent gene expression. As DOK1 gene silencing was found to be related to its promoter hypermethylation in gastric cancer [11], it will be important to investigate whether these events are associated with the presence of EBV in these cancers and others.
In conclusion, the present study sheds light on the association between EBV infection and DOK1 down-regulation in B-cells. It provides novel insights into the regulation of DOK1 in viral-related carcinogenesis, and could define it as a potential cancer biomarker and an attractive target for epigenetic-based therapy.
Materials and Methods
Expression vectors
Cellular and viral genes were expressed using the retroviral vector pLXSN (Clontech, Palo Alto, CA) or the expression vector pcDNA-3 (Invitrogen). The pLXSN-LMP-1 and the mutants LMP-1AxAxA, LMP-1 378 stop, and LMP-1AxAxA/378 stop constructs have been previously described [41]. The pGL3 basic luciferase reporter (Promega) and pGL3 containing the DOK1 promoter constructs have been described previously [29], The NF-κB super-repressor Δ-IκBα, which lacks the coding sequence of the first 36 N-terminal amino-acids, was kindly provided by Dr Elliot Kieff (Harvard Medical School, Boston, Massachusetts, USA). The expression plasmids pDEST-myc-EBNA1, pSG5-EBNA2, pDEST-myc-EBN3A1, pDEST-myc-EBNA3B, pDEST-myc-EBNA3C were kindly provided by Dr Evelyne Manet (ENS, Lyon, France).
Cells, transfection, and chemicals
RPMI 8226 cells were kindly provided by Dr Christophe Caux (Centre Léon Bérard, Lyon, France). The EBV-negative immortalized B-cells, BJAB were previously described [42], and the Louckes cells were kindly provided by Dr Evelyne Manet (ENS, Lyon, France). The primary B-cells were isolated from total blood of healthy donors using negative selection EasySep or RosetteSep (StemCell Technologies). Primary naive B cells and RPMI cells were infected with recombinant GFP-EBV, and GFP-EBVΔLMP-1 as described in [43], [44], [45], RPMI pLXSN-empty or pLXSN-LMP1 cell lines were generated as described previously [41]. Expression of LMP-1 wild-type, LMP-1 AxAxA , LMP1 378 stop, and LMP1 AxAxA/378 stop mutants in RPMI was achieved by transduction with recombinant retroviruses [41]. The EBV-immortalized lymphoblastoid cell lines (LCLs) were generated in this study by infecting primary B-cells isolated from different donors with recombinant EBV expressing GFP, as described previously [41]. Primary and immortalized B-cells were cultured in RPMI 1640 medium (GIBCO, Invitrogen life Technologies, Cergy-Pontoise, France) supplemented with 10% FBS, 100 U/ml penicillin G, 100 mg/ml streptomycin, 2 mM L-glutamine, and 1 mM sodium pyruvate (PAA, Pasching, Austria). Expression plasmids were transiently transfected in cells using Xtreme gene 9 reagents (Roche) according to the manufacturer's protocol.
For treatment, cells were incubated in media containing different reagents: with a final concentration of 1 µM of the NF-κB pathway inhibitor Bay11 in dimethyl sulfoxide (DMSO) for 6 hours. Inhibition of DNA methylation was performed by incubation for 4 days with 5-aza-2′-deoxycytidine (5-aza) at 1 µM (Sigma) dissolved in DMSO. Cells were then harvested for analysis.
Quantitative RT-PCR
Total RNA was extracted using TRIzol reagent (Life Technologies). Reverse transcription was performed using the RevertAid H Minus First Strand cDNA synthesis kit (Fermentas) according to the manufacturer's protocol. Real-time PCR was performed using the following gene-specific primers:
DOK1: Fw ATGGACGGAGCAGTGATGGA, Rev CCCAGGTCTTCCTCCACCTC
LMP1: Fw CCCCCTCTCCTCTTCCATAG, Rev GCCAAAGATGAACAGCACAA
EBNA1: Fw GGACCCGGCCCACAACCTG, Rev CTCCTGCCCTTCCTCACCCTCATC
GAPDH: Fw GAAGGTGAAGGTCGGAGTC, Rev AAGATGGTGATGGGATTTC. Data were analyzed using the ΔΔCT method.
Antibodies and immunoblotting
The following antibodies were used: anti-DOK1 (ab8112, Abcam), anti-E2F1 (KH-95; Santa Cruz Biotechnology), anti- β-Actin C4 (MP Biomedicals), anti-LMP1 (S12), anti- phosphor IκBα (#9246, Cell Signaling Technology), anti-total IκBα (#9242, Cell Signaling Technology), mouse IgG, rabbit IgG (Santa Cruz Biotechnology), anti-p65 (#3034, Cell Signaling Technology), anti-H3K4me3, and anti-H3K27me3 (Epigentek), anti-EZH2 (AC22; Cell Signaling Technology), anti-pRB (4H1, Cell Signaling Technology), anti-DNMT1 (60B1220, Abnova), anti-EBNA1 (1EB12, Santa Cruz Biotechnology), anti-EBNA2 (Novocastra), anti-EBNA3A (Exalpha), anti-EBNA3C (ab16128, Abcam). Immunoblotting was performed as described previously [29].
Reporter assays
Cells were transfected with 0.250 µg of pGL3 or DOK1 promoter constructs along with other experimental plasmids using X-tremeGENE 9 (Roche Diagnostics). The Renilla construct was included for normalization of transfection efficiency. At 48 hours after transfection, cells were harvested and the enzyme activities of firefly and Renilla luciferases were measured using the Dual-Luciferase reporter assay system (Promega). The luminescence signal was quantified using an Optocomp I luminometer (MGM Instruments). Each condition was used in triplicate and replicated in different independent experiments.
Chromatin immuno-precipitation (ChIP)
For each reaction, 106 cells were cross-linked with 1% formaldehyde, harvested and subjected to sonication to shear the chromatin into fragments of 0.2 kb, immuno-precipitated with 2 µg of appropriate antibody, and then processed according to the standard protocol for ChIP analysis from Cell Signaling Technology.
Low cell ChIP kit (Diagenode) was used for primary B cells and infected with EBV for 48 hours. 50 000 cells per reaction were processed according to the manufacturer's protocol.
The input and immuno-precipitated DNA from both methods (standard and low cell) were then analyzed by real-time PCR using primers flanking the E2F-response element (−498/−486) of the DOK1 promoter: Fw GCCAAAACCGAGGACTTTCG, Rev CATCACTGCTCCGTCCATGG, or primers for GAPDH promoter: Fw GACGGCCGCATCTTCTTGT, Rev CCTGGTGACCAGGCGC. Data were calculated as a percentage of enrichment of input.
Re-ChIP assay
Following the initial anti-E2F1 ChIP (performed as above using 107 cells and 10 µg of anti E2F1 KH-95 antibody), up to the final wash step with TE buffer, E2F1–chromatin complexes were eluted by the addition of 10 mM dithiothreitol (DTT) and incubated for 30 minutes at 37°C. Supernatants were diluted 1∶20 with re-ChIP buffer (1% Triton X-100; 20 mM Tris–HCl, pH 8.1; 2 mM EDTA; 150 mM NaCl; supplemented with protease inhibitors), and immuno-precipitated a second time (IP 2) using 4 µg of antibody against pRB, DNMT1, and EZH2. IgG was used as negative control. The Re-ChIP mixtures were incubated overnight at 4°C with rotation. Isolation and purification of associated DNA were carried out as described for the standard ChIP experiment. The binding of each factor was determined by real-time PCR as previously described. Data were calculated as a percentage of enrichment of total input.
DNA pull-down assay
Cells were lysed by sonication in HKMG buffer (10 mM HEPES, pH 7.9; 100 mM KCl; 5 mM MgCl2; 10% glycerol; 1 mM dithiothreitol (DTT); and 0.5% NP-40) containing protease and phosphatase inhibitors. Cellular debris was removed by centrifugation. Then, 1 mg of total lysate was pre-cleared with 40 µl of streptavidin-agarose beads (Thermo Scientific) for 1 hour at 4°C, with rotation, and incubated with 2 µg of biotinylated PCR product oligonucleotides and 20 µg of poly (dI-dC) for 16 hours at 4°C, with rotation. Biotin-oligonucleotide-protein complexes were collected with 60 µl of streptavidin-agarose beads for 1 hour at 4°C, with rotation, washed twice with HKMG buffer, separated on SDS-PAGE, and detected by western blotting. The biotinylated double-stranded oligonucleotides were amplified using the same primers as for ChIP with 5′ biotin.
DNA extraction and pyrosequencing
Genomic DNA was extracted using the QIAamp DNA minikit (Qiagen) and bisulfite converted using the EZ DNA Methylation-Gold kit (Zymo Research). Converted DNA was then subjected to Pyrosequencing (Qiagen) as previously described [46]. The primers used to measure the methylation of DOK1 promoter were: Fw GAGGTGGAGGAAGATTTG, Rev BIOTIN-CCACACTCACACACTCAA, and sequencing primer AGTTTTGGGGGTGGT. The percentage of methylation was evaluated as the mean of each CpG analyzed.
Flow cytometry analysis
To determine cell cycle profile, cells were collected 48 hours post-transfection with empty pCDNA3 (Vector) or expression vector pCDNA3-Flag-DOK1, washed twice with PBS 1×, and then cell pellets were re-suspended in 70% ethanol while vortexing, in order to prevent cell clumps. After ethanol fixation (30 minutes at 4°C) the cells were rewashed in PBS 1× and finally re-suspended in PBS 1×+ 100 µg/mL RNAse (Roche) + 25 µg/mL of Propidium iodide (Sigma).
Apoptotic cells were detected using the PE Annexin V apoptosis detection kit I (BD Pharmingen) according to the manufacturer's instructions.
Stained cells for cell cycle and for apoptosis were detected using the BD FACSCanto II flow cytometer (BD Biosciences) and analyzed using FACSDiva software.
Ethics statement
Blood samples from healthy donors were provided by the Etablissement Français du Sang (EFS, Lyon, France) after being anonymized. All participants signed a written informed consent.
Supporting Information
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