YTHDF1 promotes mRNA degradation via YTHDF1‐AGO2 interaction and phase separation

OBJECTIVES: YTHDF1 is known as a m(6)A reader protein, and many researches of YTHDF1 focused on the regulation of mRNA translation efficiency. However, YTHDF1 is also related to RNA degradation, but how YTHDF1 regulates mRNA degradation is indefinite. Liquid‐liquid phase separation (LLPS) underlies...

Descripción completa

Detalles Bibliográficos
Autores principales: Li, Jiong, Chen, Ke, Dong, Xin, Xu, Yating, Sun, Qi, Wang, Honghong, Chen, Zhen, Liu, Cong, Liu, Rong, Yang, Zhe, Mei, Xiangfei, Zhang, Rongyu, Chang, Liuping, Tian, Zongwen, Chen, Jianjun, Liang, Kaiwei, He, Chunjiang, Luo, Mengcheng
Formato: Online Artículo Texto
Lenguaje:English
Publicado: John Wiley and Sons Inc. 2021
Materias:
Original Articles
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8780909/
https://www.ncbi.nlm.nih.gov/pubmed/34821414
http://dx.doi.org/10.1111/cpr.13157
_version_ 1784637959017857024
author Li, Jiong
Chen, Ke
Dong, Xin
Xu, Yating
Sun, Qi
Wang, Honghong
Chen, Zhen
Liu, Cong
Liu, Rong
Yang, Zhe
Mei, Xiangfei
Zhang, Rongyu
Chang, Liuping
Tian, Zongwen
Chen, Jianjun
Liang, Kaiwei
He, Chunjiang
Luo, Mengcheng
author_facet Li, Jiong
Chen, Ke
Dong, Xin
Xu, Yating
Sun, Qi
Wang, Honghong
Chen, Zhen
Liu, Cong
Liu, Rong
Yang, Zhe
Mei, Xiangfei
Zhang, Rongyu
Chang, Liuping
Tian, Zongwen
Chen, Jianjun
Liang, Kaiwei
He, Chunjiang
Luo, Mengcheng
author_sort Li, Jiong
collection PubMed
description OBJECTIVES: YTHDF1 is known as a m(6)A reader protein, and many researches of YTHDF1 focused on the regulation of mRNA translation efficiency. However, YTHDF1 is also related to RNA degradation, but how YTHDF1 regulates mRNA degradation is indefinite. Liquid‐liquid phase separation (LLPS) underlies the formation of membraneless compartments in mammal cells, and there are few reports focused on the correlation of RNA degradation with LLPS. In this research, we focused on the mechanism of YTHDF1 degraded mRNA through LLPS. MATERIALS AND METHODS: The CRISPR/Cas9 knock out system was used to establish the YTHDF1 knock out (YTHDF1‐KO) cell lines (HEK293 and HeLa) and METTL14 knock out (METTL14‐KO) cell line (HEK293). 4SU‐TT‐seq was used to check the half‐life changes of mRNAs. Actinomycin D and qPCR were used to test the half‐life changes of individual mRNA. RNA was stained with SYTO RNA‐select dye in wild type (WT) and YTHDF1‐KO HeLa cell lines. Co‐localization of YTHDF1 and AGO2 was identified by immunofluorescence. The interaction domain of YTHDF1 and AGO2 was identified by western blot. Phase separation of YTHDF1 was performed in vitro and in vivo. Fluorescence recovery after photobleaching (FRAP) was performed on droplets as an assessment of their liquidity. RESULTS: In this research, we found that deletion of YTHDF1 led to massive RNA patches deposited in cytoplasm. The results of 4SU‐TT‐seq showed that deletion of YTHDF1 would prolong the half‐life of mRNAs. Immunofluorescence data showed that YTHDF1 and AGO2 could co‐localize in P‐body, and Co‐IP results showed that YTHDF1 could interact with AGO2 through YT521‐B homology (YTH) domain. We confirmed that YTHDF1 could undergo phase separation in vitro and in vivo, and compared with AGO2, YTHDF1 was more important in P‐body formation. The FRAP results showed that liquid AGO2 droplets would convert to gel/solid when YTHDF1 was deleted. As AGO2 plays important roles in miRISCs, we also found that miRNA‐mediate mRNA degradation is related to YTHDF1. CONCLUSIONS: YTHDF1 recruits AGO2 through the YTH domain. YTHDF1 degrades targeting mRNAs by promoting P‐body formation through LLPS. The deletion of YTHDF1 causes the P‐body to change from liquid droplets to gel/solid droplets, and form AGO2/RNA patches, resulting in a degradation delay of mRNAs. These findings reveal a previously unrecognized crosstalk between YTHDF1 and AGO2, raising a new sight of mRNA post‐transcriptional regulation by YTHDF1.
format Online
Article
Text
id pubmed-8780909
institution National Center for Biotechnology Information
language English
publishDate 2021
publisher John Wiley and Sons Inc.
record_format MEDLINE/PubMed
spelling pubmed-87809092022-02-01 YTHDF1 promotes mRNA degradation via YTHDF1‐AGO2 interaction and phase separation Li, Jiong Chen, Ke Dong, Xin Xu, Yating Sun, Qi Wang, Honghong Chen, Zhen Liu, Cong Liu, Rong Yang, Zhe Mei, Xiangfei Zhang, Rongyu Chang, Liuping Tian, Zongwen Chen, Jianjun Liang, Kaiwei He, Chunjiang Luo, Mengcheng Cell Prolif Original Articles OBJECTIVES: YTHDF1 is known as a m(6)A reader protein, and many researches of YTHDF1 focused on the regulation of mRNA translation efficiency. However, YTHDF1 is also related to RNA degradation, but how YTHDF1 regulates mRNA degradation is indefinite. Liquid‐liquid phase separation (LLPS) underlies the formation of membraneless compartments in mammal cells, and there are few reports focused on the correlation of RNA degradation with LLPS. In this research, we focused on the mechanism of YTHDF1 degraded mRNA through LLPS. MATERIALS AND METHODS: The CRISPR/Cas9 knock out system was used to establish the YTHDF1 knock out (YTHDF1‐KO) cell lines (HEK293 and HeLa) and METTL14 knock out (METTL14‐KO) cell line (HEK293). 4SU‐TT‐seq was used to check the half‐life changes of mRNAs. Actinomycin D and qPCR were used to test the half‐life changes of individual mRNA. RNA was stained with SYTO RNA‐select dye in wild type (WT) and YTHDF1‐KO HeLa cell lines. Co‐localization of YTHDF1 and AGO2 was identified by immunofluorescence. The interaction domain of YTHDF1 and AGO2 was identified by western blot. Phase separation of YTHDF1 was performed in vitro and in vivo. Fluorescence recovery after photobleaching (FRAP) was performed on droplets as an assessment of their liquidity. RESULTS: In this research, we found that deletion of YTHDF1 led to massive RNA patches deposited in cytoplasm. The results of 4SU‐TT‐seq showed that deletion of YTHDF1 would prolong the half‐life of mRNAs. Immunofluorescence data showed that YTHDF1 and AGO2 could co‐localize in P‐body, and Co‐IP results showed that YTHDF1 could interact with AGO2 through YT521‐B homology (YTH) domain. We confirmed that YTHDF1 could undergo phase separation in vitro and in vivo, and compared with AGO2, YTHDF1 was more important in P‐body formation. The FRAP results showed that liquid AGO2 droplets would convert to gel/solid when YTHDF1 was deleted. As AGO2 plays important roles in miRISCs, we also found that miRNA‐mediate mRNA degradation is related to YTHDF1. CONCLUSIONS: YTHDF1 recruits AGO2 through the YTH domain. YTHDF1 degrades targeting mRNAs by promoting P‐body formation through LLPS. The deletion of YTHDF1 causes the P‐body to change from liquid droplets to gel/solid droplets, and form AGO2/RNA patches, resulting in a degradation delay of mRNAs. These findings reveal a previously unrecognized crosstalk between YTHDF1 and AGO2, raising a new sight of mRNA post‐transcriptional regulation by YTHDF1. John Wiley and Sons Inc. 2021-11-25 /pmc/articles/PMC8780909/ /pubmed/34821414 http://dx.doi.org/10.1111/cpr.13157 Text en © 2021 The Authors. Cell Proliferation published by John Wiley & Sons Ltd. https://creativecommons.org/licenses/by/4.0/This is an open access article under the terms of the http://creativecommons.org/licenses/by/4.0/ (https://creativecommons.org/licenses/by/4.0/) License, which permits use, distribution and reproduction in any medium, provided the original work is properly cited.
spellingShingle Original Articles
Li, Jiong
Chen, Ke
Dong, Xin
Xu, Yating
Sun, Qi
Wang, Honghong
Chen, Zhen
Liu, Cong
Liu, Rong
Yang, Zhe
Mei, Xiangfei
Zhang, Rongyu
Chang, Liuping
Tian, Zongwen
Chen, Jianjun
Liang, Kaiwei
He, Chunjiang
Luo, Mengcheng
YTHDF1 promotes mRNA degradation via YTHDF1‐AGO2 interaction and phase separation
title YTHDF1 promotes mRNA degradation via YTHDF1‐AGO2 interaction and phase separation
title_full YTHDF1 promotes mRNA degradation via YTHDF1‐AGO2 interaction and phase separation
title_fullStr YTHDF1 promotes mRNA degradation via YTHDF1‐AGO2 interaction and phase separation
title_full_unstemmed YTHDF1 promotes mRNA degradation via YTHDF1‐AGO2 interaction and phase separation
title_short YTHDF1 promotes mRNA degradation via YTHDF1‐AGO2 interaction and phase separation
title_sort ythdf1 promotes mrna degradation via ythdf1‐ago2 interaction and phase separation
topic Original Articles
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8780909/
https://www.ncbi.nlm.nih.gov/pubmed/34821414
http://dx.doi.org/10.1111/cpr.13157
work_keys_str_mv AT lijiong ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT chenke ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT dongxin ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT xuyating ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT sunqi ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT wanghonghong ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT chenzhen ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT liucong ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT liurong ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT yangzhe ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT meixiangfei ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT zhangrongyu ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT changliuping ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT tianzongwen ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT chenjianjun ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT liangkaiwei ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT hechunjiang ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation
AT luomengcheng ythdf1promotesmrnadegradationviaythdf1ago2interactionandphaseseparation

Ejemplares similares