Reciprocal transactivation of Merkel cell polyomavirus and high-risk human papillomavirus promoter activities and increased expression of their oncoproteins

Papillomaviridae and Polyomaviridae are two families of non-enveloped, double-stranded DNA viruses that can cause cancer in humans [1]. High-risk human papillomaviruses (HR-HPV) are predominantly associated with cervical cancer, but also with penile, anal, vulvar, vaginal and oropharyngeal cancers [2‐10]. HR-HPV16 and HR-HPV18 are responsible for almost 70% of cervical cancers worldwide, and integration of the viral genome is considered one of the most important risk factors for cervical cancer development [5].The oncogenic potentials of HR-HPVs mainly depend on their oncoproteins E6 and E7. These proteins can bind p53 and pRb family members, respectively, but can also interfere with other hallmarks of viral oncogenesis [11‐13]. Merkel cell polyomavirus is an etiological factor for Merkel cell carcinoma (MCC), which is an aggressive skin cancer [14]. Approximately 80% of all MCC are positive for MCPyV DNA [15], and similarly to HR-HPV in cervical cancer, the MCPyV genome is integrated into all virus-positive MCC examined so far [16, 17]. The viral oncoproteins of MCPyV are denoted as large tumor antigen (LT) and small tumor antigen (sT) [18, 19]. Equivalently, as seen in HPV, LT can interfere with the activity of p53 and pRb proteins [19, 20].This similar effect also suggests that E6, E7 and LT may act together to augment the transformative properties of HR-HPV in cells were co-infection occurs.

Co-infection of human polyomaviruses in HR-HPV positive tumors has been reported, underscoring the possibility that human polyomaviruses can act as a co-factor in HR-HPV-induced oncogenesis. Co-presence of BK polyomavirus (BKPyV) and HR-HPV has been reported in oropharyngeal malignancies, cervical swabs, and genital tumors [2, 21‐25]. BKPyV DNA or JC polyomavirus DNA was detected in HR-HPV positive precancerous cervical lesions and in oropharyngeal squamous cell carcinomas [22, 26, 27]. However, whether these polyomavirus have an impact on cancer development remains unknown.

In cervical tumor samples, MCPyV DNA could be amplified in 19% of HR-HPV positive cervical squamous cell carcinomas (n = 48), and in 25% of HR-HPV positive cervical adenocarcinomas (n = 16) [28]. In another study, 14 out of 45 (34%) HR-HPV positive cervical tumors were also positive for MCPyV DNA [29]. Kolia-Diafouka and colleges detected HR-HPV in 124 out of 140 (88.6%) cervical samples from HIV-positive African women and in 24 out of 50 (48%) samples from HIV-negative French women. Interestingly, 81 (55%) of these 148 HR-HPV positive samples were also positive for MCPyV, but there was no significant difference with HR-HPV negative samples, of which 24/42 (57%) were MCPyV positive. There was no association between detection of human polyomaviruses in cervical specimens and HR-HPV coinfection or precancerous cervical lesions [30]. MCPyV DNA has also been observed in HR-HPV positive oropharyngeal cancers and in HR-HPV positive tonsillar SCC, but the prevalence of MCPyV DNA in benign tonsillar tissue did not differ significantly compared with malignant tissue [24, 31, 32]. These observations argue against a possible role of MCPyV as a cofactor in HPV-induced carcinogenesis.

Although a co-factor role for MCPyV in HR-HPV-induced cancers remains to be proven, the co-detection of MCPyV DNA in HR-HPV positive tumor specimens and the known oncogenic potential of MCPyV suggest that MCPyV may promote HPV-induced oncogenesis. This prompted us to investigate whether the MCPyV oncoproteins LT and sT could enhance the expression of the major HR-HPV oncoproteins E6 and E7, thereby accelerating the initiation and progression of HR-HPV-induced neoplasia. A possible effect of E6 and E7 on the transcriptional activity of MCPyV was also explored.

A causal role of HR-HPV, especially HPV16 and HPV18, in anogenital and oropharyngeal cancers is well-established [2, 3, 5‐8]. MCPyV is the etiological factor of 80% of MCC [15], but MCPyV has also been detected in oropharyngeal and anogenital tumors, but their role in these cancers is not known (reviewed in [52]). Because double infection with HR-HPV and MCPyV has been reported in anogenital and oropharyngeal cancers [24, 32], we examined whether an interaction between HR-HPV and MCPyV exists.

First, we compared the promoter activities of HPV16, HPV18 and MCPyV in three different cell lines. We found that the transcriptional activity of the HPV18 LCR was 6–10 times stronger than that of the HVP16 LCR in C33A and HaCaT cells, but comparable in HSC-3 cells (Fig. 1). Chen et al. also reported that the basal transcriptional activity of the HPV18 LCR was about three fold higher than that of HPV16 LCR in HeLa cells and in breast cancer T47D cells [53]. Ottinger et al. showed that the HPV18 LCR activity was 5–20-fold stronger than the HPV16 LCR activity in the cervical carcinoma cell lines C33A, HeLa and SiHa and in normal oral keratinocytes, but lower in African Green Monkey kidney epithelial cells CV-1 and comparable in hTERT immortalized human BJ fibroblasts [54]. The MCPyV early and late promoter activities were comparable in C33A and HaCaT cells, whereas the early promoter was approximately 40% stronger in HSC-3 cells. The early as well as the late MCPyV promoter had significantly weaker transcriptional activity than the HPV16 LCR and the HPV18 LCR in HaCaT and HSC-3 cells, but both were stronger compared to HPV16 LCR in C33A. To our best knowledge, this is the first study comparing the basal activities of the HPV16/18 LCRs and MCPyV promoter. Transient expression of MCPyV sT, full-length LT, or sT plus LT was shown to stimulate the transcriptional activity of the HPV16 and HPV18 LCR in C33A and HSC-3 cells, whereas LT induced HPV16 LCR and HPV18 LCR activity in HaCaT cells, but not sT, which significantly reduced the activity of these LCRs in HaCaT cells (Fig. 2). These results suggest a cell-specific effect of LT and sT on the LCR activity of HPV16 and HPV18. Previous studies with the HPV16 and HPV18 promoter in other cell lines showed a variable stimulating effect of LT and sT of the polyomavirus SV40. SV40 LT increased HPV18 promoter activity 13-fold in HeLa cells, ~ threefold in SW13 (human adrenocortical carcinoma) and in 3T6 (mouse fibroblasts) cells, but had no effect in monkey kidney CV-1 cells [55]. In human keratinocytes, a ninefold increase in HPV18 promoter strength was observed in the simultaneous presence of LT and sT [56]. In human embryonal fibroblasts, the HPV16 promoter activity was stimulated 20- to 30-fold by SV40 sT, while the effect of LT was 5- to sixfold weaker than sT [57]. We examined the mechanism by which MCPyV LT and sT stimulate the activity of the LCR of HPV16 and HPV18. LT can activate heterogeneous promoters by binding to adjacently repeated G^A/_GGGC motifs [58]. Yet, a sequence analysis of the HPV16 and HPV18 promoters did not reveal repeated LT binding motifs. Moreover, the C-terminal truncated LT variants MKL1 and MKL2, which lack the DNA binding domain, still activated the HPV16 and HPV18 promoters (Fig. 4A). Therefore, the nuclear presence of LT seems not necessary because the MKL2 LT variant lacks a functional NLS [42]. Mutations in LT that abrogate the binding to HSC70, pRb and to hVam6p did not impair LT-mediated trans-activation of the HPV 16 LCR and HPV18 LCR. Likewise, sT mutants defective in interacting with HSC70, PP2A, and ubiquitin ligase Fbxw7 did not abolish sT-induced stimulation of HPV16 LCR and HPV18 LCR transcriptional activity (Fig. 4B, C). The exact mechanism by which the MCPyV oncoproteins stimulate HVP16 and HPV18 LCR activity remains unknown. LT and sT can affect different signaling pathways [19, 59], which may regulate the activity of transcription factors that control the transcriptional activity of these LCRs. The exact sequences required for LT- and sT-mediated activation of the HPV16 LCR and HPV18 LCR could not be determined by truncation versions of these LCRs because the transcriptional activity of truncated LCRs was still induced by LT and sT. Further studies are required to map the exact LCR sequences that mediate LT- and sT-induced activation. The LCR of the HPV16 and HPV18 contain binding motifs for several transcription factors, including AP1, NF1, YY1, SP1, OCT-1, TEF-1, C/EBPβ, STAT3, glucocorticoid/progesterone receptor, FOXA1, MYC, and some distinctive ones such as SOX2 and FOXA-2 for HPV16 LCR and GATA3 and TFAB2B for HPV18 LCR [60‐62], but it remains to be determined whether these are implicated in LT- or sT-triggered activation of the HPV16/18 LCR. MCPyV LT and sT can interact with several proteins involved in signaling and transcription (reviewed in [19]), but the biological roles of these interactions are unknown. Stimulation of the MCPyV early and late promoters by E6 and E7 was only affected by the E6 F47R mutant. This E6 mutant, which counteracts p53 degradation mediated by wild-type E6 [48], failed or had reduced ability to stimulate the MCPyV early and late promoter. However, the E6 C106R mutant, which cannot bind p53, increased MCPyV early and late promoter activity comparable to wild-type E6. More than 50 different cellular proteins interact with E6 [11, 13], but whether the F47R mutation disrupts such interaction(s) thereby affecting E6’s ability to trans-activate the MCPyV promoters remains to be established.

Our results show that the oncoproteins LT and sT from MCPyV can stimulate the transcriptional activity of the HPV16 LCR and the HPV18 LCR and induce expression of proteins from these LCR. On the other hand, the E6 and E7 oncoproteins of HR-HPV can trans-activate the MCPyV early and late promoter and augment expression of the MCPyV LT oncoprotein. The exact mechanism for this reciprocal trans-activation remains elusive. Co-infection with HR-HPV and MCPyV may enhance the oncogenic potentials of these viruses through reciprocal potentiating the expression levels of their oncoproteins.