National Institute of Biomedical Genomics, P.O.: N.S.S, Kalyani, 741251, West Bengal, India.
Tata Medical Center, Kolkata, West Bengal, India.
Clin Epigenetics. 2024 Mar 10;16(1):40. doi: 10.1186/s13148-024-01651-9.
MAL (T-lymphocyte maturation-associated protein) is highly downregulated in most cancers, including cervical cancer (CaCx), attributable to promoter hypermethylation. Long noncoding RNA genes (lncGs) play pivotal roles in CaCx pathogenesis, by interacting with human papillomavirus (HPV)-encoded oncoproteins, and epigenetically regulating coding gene expression. Hence, we attempted to decipher the impact and underlying mechanisms of MAL downregulation in HPV16-related CaCx pathogenesis, by interrogating the interactive roles of MAL antisense lncRNA AC103563.8, E7 oncoprotein and PRC2 complex protein, EZH2.
Employing strand-specific RNA-sequencing, we confirmed the downregulated expression of MAL in association with poor overall survival of CaCx patients bearing HPV16, along with its antisense long noncoding RNA (lncRNA) AC103563.8. The strength of positive correlation between MAL and AC103563.8 was significantly high among patients compared to normal individuals. While downregulated expression of MAL was significantly associated with poor overall survival of CaCx patients bearing HPV16, AC103563.8 did not reveal any such association. We confirmed the enrichment of chromatin suppressive mark, H3K27me3 at MAL promoter, using ChIP-qPCR in HPV16-positive SiHa cells. Subsequent E7 knockdown in such cells significantly increased MAL expression, concomitant with decreased EZH2 expression and H3K27me3 marks at MAL promoter. In silico analysis revealed that both E7 and EZH2 bear the potential of interacting with AC103563.8, at the same binding domain. RNA immunoprecipitation with anti-EZH2 and anti-E7 antibodies, respectively, and subsequent quantitative PCR analysis in E7-silenced and unperturbed SiHa cells confirmed the interaction of AC103563.8 with EZH2 and E7, respectively. Apparently, AC103563.8 seems to preclude EZH2 and bind with E7, failing to block EZH2 function in patients. Thereby, enhanced EZH2 expression in the presence of E7 could potentially inactivate the MAL promoter through H3K27me3 marks, corroborating our previous results of MAL expression downregulation in patients.
AC103563.8-E7-EZH2 axis, therefore, appears to crucially regulate the expression of MAL, through chromatin inactivation in HPV16-CaCx pathogenesis, warranting therapeutic strategy development.
MAL(T 淋巴细胞成熟相关蛋白)在大多数癌症中,包括宫颈癌(CaCx),由于启动子过度甲基化而高度下调。长链非编码 RNA 基因(lncGs)通过与人类乳头瘤病毒(HPV)编码的致癌蛋白相互作用,并通过表观遗传调节编码基因表达,在 CaCx 发病机制中发挥关键作用。因此,我们试图通过研究 MAL 反义 lncRNA AC103563.8、E7 致癌蛋白和 PRC2 复合物蛋白 EZH2 的相互作用,来解读 MAL 下调在 HPV16 相关 CaCx 发病机制中的影响和潜在机制。
通过特异性 RNA 测序,我们证实了 MAL 在 HPV16 阳性 CaCx 患者中与整体生存不良相关,并且与它的反义长链非编码 RNA(lncRNA)AC103563.8 相关。与正常个体相比,MAL 和 AC103563.8 之间的正相关强度在患者中显著较高。MAL 的下调表达与 HPV16 阳性 CaCx 患者的整体生存不良显著相关,而 AC103563.8 则没有显示出这种相关性。我们使用 ChIP-qPCR 在 HPV16 阳性 SiHa 细胞中证实了 MAL 启动子处染色质抑制标记 H3K27me3 的富集。随后在这些细胞中敲低 E7,显著增加了 MAL 的表达,同时降低了 MAL 启动子处的 EZH2 表达和 H3K27me3 标记。计算机分析表明,E7 和 EZH2 都具有与 AC103563.8 相互作用的潜力,在同一结合域。用抗 EZH2 和抗 E7 抗体进行 RNA 免疫沉淀,然后在 E7 沉默和未处理的 SiHa 细胞中进行定量 PCR 分析,分别证实了 AC103563.8 与 EZH2 和 E7 的相互作用。显然,AC103563.8 似乎可以阻止 EZH2 与 E7 结合,从而无法阻止 EZH2 在患者中的功能。因此,在存在 E7 的情况下,增强的 EZH2 表达可能通过 H3K27me3 标记使 MAL 启动子失活,这与我们之前在患者中 MAL 表达下调的结果一致。
因此,AC103563.8-E7-EZH2 轴似乎通过 HPV16-CaCx 发病机制中的染色质失活,关键调节 MAL 的表达,值得开发治疗策略。
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