Epitranscriptomics M<sup>6</Sup>a Analyses Reveal Distinct M<sup>6</Sup>a Marks Under Tumor Necrosis Factor Α (tnf-Α) Apoptotic Conditions in Hela Cells
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Date
2024
Authors
Tüncel, Özge
Akgül, Bünyamin
Journal Title
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Volume Title
Publisher
Wiley
Open Access Color
HYBRID
Green Open Access
Yes
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Publicly Funded
No
Abstract
Tumor necrosis factor-alpha (TNF-alpha) is a ligand that induces both intrinsic and extrinsic apoptotic pathways in HeLa cells by modulating complex gene regulatory mechanisms. However, the full spectrum of TNF-alpha-modulated epitranscriptomic m(6)A marks is unknown. We employed a genomewide approach to examine the extent of m(6)A RNA modifications under TNF-alpha-modulated apoptotic conditions in HeLa cells. miCLIP-seq analyses revealed a plethora of m(6)A marks on 632 target mRNAs with an enrichment on 99 mRNAs associated with apoptosis. Interestingly, the m(6)A RNA modification patterns were quite different under cisplatin- and TNF-alpha-mediated apoptotic conditions. We then examined the abundance and translational efficiencies of several mRNAs under METTL3 knockdown and/or TNF-alpha treatment conditions. Our analyses showed changes in the translational efficiency of TP53INP1 mRNA based on the polysome profile analyses. Additionally, TP53INP1 protein amount was modulated by METTL3 knockdown upon TNF-alpha treatment but not CP treatment, suggesting the existence of a pathway-specific METTL3-TP53INP1 axis. Congruently, METLL3 knockdown sensitized HeLa cells to TNF-alpha-mediated apoptosis, which was also validated in a zebrafish larval xenograft model. These results suggest that apoptotic pathway-specific m(6)A methylation marks exist in cells and TNF-alpha-METTL3-TP53INP1 axis modulates TNF-alpha-mediated apoptosis in HeLa cells.
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Keywords
apoptosis, epitranscriptomics, Hela, m6A, RNA modification, TNF-alpha, Gene Expression Regulation, Tumor Necrosis Factor-alpha, Animals, Humans, Apoptosis, Methyltransferases, RNA, Messenger, Carrier Proteins, Heat-Shock Proteins, Zebrafish, HeLa Cells, Epigenesis, Genetic
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Q1
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Q1

OpenCitations Citation Count
3
Source
Journal of Cellular Physiology
Volume
239
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Scopus : 5
PubMed : 3
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