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Targeting histone deacetylase suppresses tumor growth through eliciting METTL14‐modified m6A RNA methylation in ocular melanoma

癌症研究 核糖核酸 生物 分子生物学 组蛋白 组蛋白脱乙酰基酶 DNA甲基化 RNA甲基化 化学 黑色素瘤 医学 DNA 基因表达 甲基转移酶 甲基化 生物化学 基因
作者
Ai Zhuang,Xiang Gu,Tongxin Ge,Shaoyun Wang,Shengfang Ge,Peiwei Chai,Renbing Jia,Xianqun Fan
出处
期刊:Cancer communications [Wiley]
卷期号:43 (11): 1185-1206 被引量:8
标识
DOI:10.1002/cac2.12471
摘要

Abstract Background Diversified histone deacetylation inhibitors (HDACis) have demonstrated encouraging outcomes in multiple malignancies. N6‐methyladenine (m 6 A) is the most prevalent messenger RNA modification that plays an essential role in the regulation of tumorigenesis. Howbeit, an in‐depth understanding of the crosstalk between histone acetylation and m 6 A RNA modifications remains enigmatic. This study aimed to explore the role of histone acetylation and m 6 A modifications in the regulation of tumorigenesis of ocular melanoma. Methods Histone modification inhibitor screening was used to explore the effects of HDACis on ocular melanoma cells. Dot blot assay was used to detect the global m 6 A RNA modification level. Multi‐omics assays, including RNA‐sequencing, cleavage under targets and tagmentation, single‐cell sequencing, methylated RNA immunoprecipitation‐sequencing (meRIP‐seq), and m 6 A individual nucleotide resolution cross‐linking and immunoprecipitation‐sequencing (miCLIP‐seq), were performed to reveal the mechanisms of HDACis on methyltransferase‐like 14 ( METTL14 ) and FAT tumor suppressor homolog 4 ( FAT4 ) in ocular melanoma. Quantitative real‐time polymerase chain reaction (qPCR), western blotting, and immunofluorescent staining were applied to detect the expression of METTL14 and FAT4 in ocular melanoma cells and tissues. Cell models and orthotopic xenograft models were established to determine the roles of METTL14 and FAT4 in the growth of ocular melanoma. RNA‐binding protein immunoprecipitation‐qPCR, meRIP‐seq, miCLIP‐seq, and RNA stability assay were adopted to investigate the mechanism by which m 6 A levels of FAT4 were affected. Results First, we found that ocular melanoma cells presented vulnerability towards HDACis. HDACis triggered the elevation of m 6 A RNA modification in ocular melanoma. Further studies revealed that METTL14 served as a downstream candidate for HDACis. METTL14 was silenced by the hypo‐histone acetylation status, whereas HDACi restored the normal histone acetylation level of METTL14 , thereby inducing its expression. Subsequently, METTL14 served as a tumor suppressor by promoting the expression of FAT4 , a tumor suppressor, in a m 6 A‐YTH N6‐methyladenosine RNA‐binding protein 1‐dependent manner. Taken together, we found that HDACi restored the histone acetylation level of METTL14 and subsequently elicited METTL14‐mediated m 6 A modification in tumorigenesis. Conclusions These results demonstrate that HDACis exert anti‐cancer effects by orchestrating m 6 A modification, which unveiling a “histone‐RNA crosstalk” of the HDAC/ METTL14 / FAT4 epigenetic cascade in ocular melanoma.
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