[No authors listed]
Breast cancer (BC) is the most frequently diagnosed cancer and the leading cause of cancerârelated death among women worldwide. Evidence indicates that posttranscriptional N6âmethyladenosine (m6A) modification modulates BC development. In the present study, we assessed BC and normal tissues to investigate this connection. RNA m6A levels were determined by methylation quantification assay. The effects of methyltransferaseâlike 14 (METTL14) gainâofâexpression or coâtransfection with an m6A inhibitor on cell migration and invasion abilities were determined by Transwell assays. The levels of differentially expressed (DE) miRNAs were verified by realâtime quantitative PCR (RTâqPCR). Gene Ontology (GO) and Kyoto Encyclopedia of Genes and Genomes analyses (KEGG) were performed to analyze potential function of target genes of the DE miRNAs. The effects of candidate miRNAs modulated by METTL14 on cell migration and invasion abilities were confirmed by Transwell assays. We demonstrated that m6A methyltransferase METTL14 was significantly upregulated in BC tissues compared with normal tissues. METTL14 gainâ and lossâofâexpression regulated m6A levels in MCFâ7 and MDAâMBâ231 cells. The cell function assays revealed that METTL14 overexpression enhanced the migration and invasion capacities of BC cells. Moreover, treatment with the m6A inhibitor suppressed this enhanced cell migration and invasion. Additionally, aberrant expression of METTL14 reshaped the miRNA profile in BC cell lines. The remodeled DE miRNA/mRNA network was found to be most enriched in cancer pathways, and DE miRNAs were enriched in cell adhesion terms. hsaâmiRâ146aâ5p modulated by METTL14 promoted cell migration and invasion. METTL14 modulates m6A modification and hsaâmiRâ146aâ5p expression, thereby affecting the migration and invasion of breast cancer cells.
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