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HMGA1a Induces Alternative Splicing of the Estrogen Receptor-αlpha Gene by Trapping U1 snRNP to an Upstream Pseudo-5′ Splice Site

Objectives: The high-mobility group A protein 1a (HMGA1a) protein is known as a transcription factor that binds to DNA, but recent studies have shown it exerts novel functions through RNA-binding. We were prompted to decipher the mechanism of HMGA1a-induced alternative splicing of the estrogen recep...

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Autores principales: Ohe, Kenji, Miyajima, Shinsuke, Tanaka, Tomoko, Hamaguchi, Yuriko, Harada, Yoshihiro, Horita, Yuta, Beppu, Yuki, Ito, Fumiaki, Yamasaki, Takafumi, Terai, Hiroki, Mori, Masayoshi, Murata, Yusuke, Tanabe, Makito, Abe, Ichiro, Ashida, Kenji, Kobayashi, Kunihisa, Enjoji, Munechika, Nomiyama, Takashi, Yanase, Toshihiko, Harada, Nobuhiro, Utsumi, Toshiaki, Mayeda, Akila
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Frontiers Media S.A. 2018
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6002489/
https://www.ncbi.nlm.nih.gov/pubmed/29938207
http://dx.doi.org/10.3389/fmolb.2018.00052
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author Ohe, Kenji
Miyajima, Shinsuke
Tanaka, Tomoko
Hamaguchi, Yuriko
Harada, Yoshihiro
Horita, Yuta
Beppu, Yuki
Ito, Fumiaki
Yamasaki, Takafumi
Terai, Hiroki
Mori, Masayoshi
Murata, Yusuke
Tanabe, Makito
Abe, Ichiro
Ashida, Kenji
Kobayashi, Kunihisa
Enjoji, Munechika
Nomiyama, Takashi
Yanase, Toshihiko
Harada, Nobuhiro
Utsumi, Toshiaki
Mayeda, Akila
author_facet Ohe, Kenji
Miyajima, Shinsuke
Tanaka, Tomoko
Hamaguchi, Yuriko
Harada, Yoshihiro
Horita, Yuta
Beppu, Yuki
Ito, Fumiaki
Yamasaki, Takafumi
Terai, Hiroki
Mori, Masayoshi
Murata, Yusuke
Tanabe, Makito
Abe, Ichiro
Ashida, Kenji
Kobayashi, Kunihisa
Enjoji, Munechika
Nomiyama, Takashi
Yanase, Toshihiko
Harada, Nobuhiro
Utsumi, Toshiaki
Mayeda, Akila
author_sort Ohe, Kenji
collection PubMed
description Objectives: The high-mobility group A protein 1a (HMGA1a) protein is known as a transcription factor that binds to DNA, but recent studies have shown it exerts novel functions through RNA-binding. We were prompted to decipher the mechanism of HMGA1a-induced alternative splicing of the estrogen receptor alpha (ERα) that we recently reported would alter tamoxifen sensitivity in MCF-7 TAMR1 cells. Methods: Endogenous expression of full length ERα66 and its isoform ERα46 were evaluated in MCF-7 breast cancer cells by transient expression of HMGA1a and an RNA decoy (2′-O-methylated RNA of the HMGA1a RNA-binding site) that binds to HMGA1a. RNA-binding of HMGA1a was checked by RNA-EMSA. In vitro splicing assay was performed to check the direct involvement of HMGA1a in splicing regulation. RNA-EMSA assay in the presence of purified U1 snRNP was performed with psoralen UV crosslinking to check complex formation of HMGA1a-U1 snRNP at the upstream pseudo-5′ splice site of exon 1. Results: HMGA1a induced exon skipping of a shortened exon 1 of ERα in in vitro splicing assays that was blocked by the HMGA1a RNA decoy and sequence-specific RNA-binding was confirmed by RNA-EMSA. RNA-EMSA combined with psoralen UV crosslinking showed that HMGA1a trapped purified U1 snRNP at the upstream pseudo-5′ splice site. Conclusions: Regulation of ERα alternative splicing by an HMGA1a-trapped U1 snRNP complex at the upstream 5′ splice site of exon 1 offers novel insight on 5′ splice site regulation by U1 snRNP as well as a promising target in breast cancer therapy where alternative splicing of ERα is involved.
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spelling pubmed-60024892018-06-22 HMGA1a Induces Alternative Splicing of the Estrogen Receptor-αlpha Gene by Trapping U1 snRNP to an Upstream Pseudo-5′ Splice Site Ohe, Kenji Miyajima, Shinsuke Tanaka, Tomoko Hamaguchi, Yuriko Harada, Yoshihiro Horita, Yuta Beppu, Yuki Ito, Fumiaki Yamasaki, Takafumi Terai, Hiroki Mori, Masayoshi Murata, Yusuke Tanabe, Makito Abe, Ichiro Ashida, Kenji Kobayashi, Kunihisa Enjoji, Munechika Nomiyama, Takashi Yanase, Toshihiko Harada, Nobuhiro Utsumi, Toshiaki Mayeda, Akila Front Mol Biosci Molecular Biosciences Objectives: The high-mobility group A protein 1a (HMGA1a) protein is known as a transcription factor that binds to DNA, but recent studies have shown it exerts novel functions through RNA-binding. We were prompted to decipher the mechanism of HMGA1a-induced alternative splicing of the estrogen receptor alpha (ERα) that we recently reported would alter tamoxifen sensitivity in MCF-7 TAMR1 cells. Methods: Endogenous expression of full length ERα66 and its isoform ERα46 were evaluated in MCF-7 breast cancer cells by transient expression of HMGA1a and an RNA decoy (2′-O-methylated RNA of the HMGA1a RNA-binding site) that binds to HMGA1a. RNA-binding of HMGA1a was checked by RNA-EMSA. In vitro splicing assay was performed to check the direct involvement of HMGA1a in splicing regulation. RNA-EMSA assay in the presence of purified U1 snRNP was performed with psoralen UV crosslinking to check complex formation of HMGA1a-U1 snRNP at the upstream pseudo-5′ splice site of exon 1. Results: HMGA1a induced exon skipping of a shortened exon 1 of ERα in in vitro splicing assays that was blocked by the HMGA1a RNA decoy and sequence-specific RNA-binding was confirmed by RNA-EMSA. RNA-EMSA combined with psoralen UV crosslinking showed that HMGA1a trapped purified U1 snRNP at the upstream pseudo-5′ splice site. Conclusions: Regulation of ERα alternative splicing by an HMGA1a-trapped U1 snRNP complex at the upstream 5′ splice site of exon 1 offers novel insight on 5′ splice site regulation by U1 snRNP as well as a promising target in breast cancer therapy where alternative splicing of ERα is involved. Frontiers Media S.A. 2018-06-08 /pmc/articles/PMC6002489/ /pubmed/29938207 http://dx.doi.org/10.3389/fmolb.2018.00052 Text en Copyright © 2018 Ohe, Miyajima, Tanaka, Hamaguchi, Harada, Horita, Beppu, Ito, Yamasaki, Terai, Mori, Murata, Tanabe, Abe, Ashida, Kobayashi, Enjoji, Nomiyama, Yanase, Harada, Utsumi and Mayeda. http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) and the copyright owner are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
spellingShingle Molecular Biosciences
Ohe, Kenji
Miyajima, Shinsuke
Tanaka, Tomoko
Hamaguchi, Yuriko
Harada, Yoshihiro
Horita, Yuta
Beppu, Yuki
Ito, Fumiaki
Yamasaki, Takafumi
Terai, Hiroki
Mori, Masayoshi
Murata, Yusuke
Tanabe, Makito
Abe, Ichiro
Ashida, Kenji
Kobayashi, Kunihisa
Enjoji, Munechika
Nomiyama, Takashi
Yanase, Toshihiko
Harada, Nobuhiro
Utsumi, Toshiaki
Mayeda, Akila
HMGA1a Induces Alternative Splicing of the Estrogen Receptor-αlpha Gene by Trapping U1 snRNP to an Upstream Pseudo-5′ Splice Site
title HMGA1a Induces Alternative Splicing of the Estrogen Receptor-αlpha Gene by Trapping U1 snRNP to an Upstream Pseudo-5′ Splice Site
title_full HMGA1a Induces Alternative Splicing of the Estrogen Receptor-αlpha Gene by Trapping U1 snRNP to an Upstream Pseudo-5′ Splice Site
title_fullStr HMGA1a Induces Alternative Splicing of the Estrogen Receptor-αlpha Gene by Trapping U1 snRNP to an Upstream Pseudo-5′ Splice Site
title_full_unstemmed HMGA1a Induces Alternative Splicing of the Estrogen Receptor-αlpha Gene by Trapping U1 snRNP to an Upstream Pseudo-5′ Splice Site
title_short HMGA1a Induces Alternative Splicing of the Estrogen Receptor-αlpha Gene by Trapping U1 snRNP to an Upstream Pseudo-5′ Splice Site
title_sort hmga1a induces alternative splicing of the estrogen receptor-αlpha gene by trapping u1 snrnp to an upstream pseudo-5′ splice site
topic Molecular Biosciences
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6002489/
https://www.ncbi.nlm.nih.gov/pubmed/29938207
http://dx.doi.org/10.3389/fmolb.2018.00052
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