5azadC treatment upregulates miR-375 level and represses HPV16 E6 expression.

Adrien Morel,David Guenat,Elise Jacquin,Caroline Demeret,Jean-Luc Prétet,Christiane Mougin,Aurélie Baguet,Jérôme Perrard

doi:10.18632/oncotarget.17575

Abstract

High-risk human papillomaviruses are the etiological agents of cervical cancer and HPV16 is the most oncogenic genotype. Immortalization and transformation of infected cells requires the overexpression of the two viral oncoproteins E6 and E7 following HPV DNA integration into the host cell genome. Integration often leads to the loss of the E2 open reading frame and the corresponding protein can no longer act as a transcriptional repressor on p97 promoter. Recently, it has been proposed that long control region methylation also contributes to the regulation of E6/E7 expression.To determine which epigenetic mechanism is involved in HPV16 early gene regulation, 5-aza-2′-deoxycytidine was used to demethylate Ca Ski and SiHa cell DNA. Decreased expression of E6 mRNA and protein levels was observed in both cell lines in an E2-independent manner. E6 repression was accompanied by neither a modification of the main cellular transcription factor expression involved in long control region regulation, nor by a modification of the E6 mRNA splicing pattern. In contrast, a pronounced upregulation of miR-375, known to destabilize HPV16 early viral mRNA, was observed. Finally, the use of miR-375 inhibitor definitively proved the involvement of miR-375 in E6 repression. These results highlight that cellular DNA methylation modulates HPV16 early gene expression and support a role for epigenetic events in high-risk HPV associated-carcinogenesis.

Highlights

Among the 170 HPV described in 2013 [1], 12 highrisk HPV are classified as carcinogenic to humans by the IARC [2]
We showed that the treatment of HPV16 positive Ca Ski and SiHa cells with the demethylating agent 5azadC induces repression of E6 expression at both mRNA and protein levels
This cell line presents nearly 500 integrated HPV16 genomes in head-to-tail concatemers and a highly methylated long control region (LCR) (>80%), especially on the 5 CpG involved in the regulation of early viral gene expression and located in the two proximal E2 Binding Sites (E2BS) [17]

Summary

Introduction

Among the 170 HPV described in 2013 [1], 12 highrisk HPV (hrHPV) are classified as carcinogenic to humans by the IARC [2]. The HPV16 genome is a circular double-stranded DNA It harbors 8 open reading frames (ORFs) encoding early (E1, E2, E4, E5, E6 and E7) and late (L1 and L2) viral proteins and a long control region (LCR) containing transcription control sequences. The LCR presents numerous binding sites for cellular transcription factors known to activate (TATA binding protein, Sp1, AP-1 and NFI) or repress (YY1) transcription of viral early genes [6]. It exhibits four E2 Binding Sites (E2BS) with common consensus sequence 5′-ACCG(N)4CGGT-3′ and different affinities for E2 [7]. The repressor activity of E2 is linked to its ability to displace cellular transcriptional activators from their binding site due to steric hindrance [8]

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