| Literature DB >> 29678492 |
Kenji Ohe1, Shinsuke Miyajima2, Ichiro Abe3, Tomoko Tanaka4, Yuriko Hamaguchi4, Yoshihiro Harada5, Yuta Horita5, Yuki Beppu5, Fumiaki Ito5, Takafumi Yamasaki5, Hiroki Terai5, Masayoshi Mori5, Yusuke Murata5, Makito Tanabe4, Kenji Ashida6, Kunihisa Kobayashi3, Munechika Enjoji5, Toshihiko Yanase4, Nobuhiro Harada7, Toshiaki Utsumi2, Akila Mayeda8.
Abstract
The high-mobility group A protein 1a (HMGA1a) protein is known as an oncogene whose expression level in cancer tissue correlates with the malignant potential, and known as a component of senescence-related structures connecting it to tumor suppressor networks in fibroblasts. HMGA1 protein binds to DNA, but recent studies have shown it exerts novel functions through RNA-binding. Our previous studies have shown that sequence-specific RNA-binding of HMGA1a induces exon-skipping of Presenilin-2 exon 5 in sporadic Alzheimer disease. Here we show that HMGA1a induced exon-skipping of the estrogen receptor alpha (ERα) gene and increased ERα46 mRNA expression in MCF-7 breast cancer cells. An RNA-decoy of HMGA1a efficiently blocked this event and reduced ERα46 protein expression. Blockage of HMGA1a RNA-binding property consequently induced cell growth through reduced ERα46 expression in MCF-7 cells and increased sensitivity to tamoxifen in the tamoxifen-resistant cell line, MCF-7/TAMR1. Stable expression of an HMGA1a RNA-decoy in MCF-7 cells exhibited decreased ERα46 protein expression and increased estrogen-dependent tumor growth when these cells were implanted in nude mice. These results show HMGA1a is involved in alternative splicing of the ERα gene and related to estrogen-related growth as well as tamoxifen sensitivity in MCF-7 breast cancer cells.Entities:
Keywords: Breast cancer; Estrogen receptor
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Year: 2018 PMID: 29678492 DOI: 10.1016/j.jsbmb.2018.04.007
Source DB: PubMed Journal: J Steroid Biochem Mol Biol ISSN: 0960-0760 Impact factor: 4.292