Titolo | TGFβ-induced c-Myb affects the expression of EMT-associated genes and promotes invasion of ER+ breast cancer cells |
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Tipo di pubblicazione | Articolo su Rivista peer-reviewed |
Anno di Pubblicazione | 2011 |
Autori | Cesi, Vincenzo, Casciati A., Sesti F., Tanno Barbara, Calabretta B., and Raschellà G. |
Rivista | Cell Cycle |
Volume | 10 |
Paginazione | 4149-4161 |
ISSN | 15384101 |
Parole chiave | 3' untranslated region, Apoptosis, article, Breast cancer, cancer cell, cancer invasion, cell anchorage, Cell Count, cell growth, cell invasion, cell strain MCF 7, controlled study, down regulation, enzyme activity, epithelial mesenchymal transition, estrogen receptor, etoposide, Female, gene mapping, gene silencing, gene vector, genetic transcription, genetic transfection, half life time, human, human cell, luciferase, microRNA, microRNA 200b, microRNA 200c, microRNA 429, molecular mechanics, protein bcl 2, protein c Myb, protein expression, protein function, protein stability, RNA binding, transforming growth factor beta, transforming growth factor beta receptor 1, unclassified drug, uvomorulin |
Abstract | Advanced breast cancer cells acquire metastatic properties in response to TGFβ. We show here that the expression of c-Myb increases in TGFβ-treated ER+ breast cancer cells by protein stabilization, transcription activation and release from miR200-dependent downregulation. In particular, we mapped two sites for miR200b, miR200c and miR429 binding in the 3′ UTR of the human c-myb gene. These microRNAs decreased the expression of c-Myb when transfected in MCF-7 cells. In addition, luciferase activity from a vector containing the 3′ UTR of the c-myb gene was inhibited by miR200s through a binding-dependent mechanism. siRNA- and shRNA-mediated downregulation was used to investigate the role of c-Myb for the effects induced by TGFβ in ER+ breast cancer MCF-7 and ZR-75.1 cells. Transfection with c-Myb siRNAs blocked the increase of Slug (SNAI2) and Bcl-2 expression and reversed the decrease in E-cadherin expression induced by TGFβ treatment. Conversely, c-Myb downregulation decreased invasion and anchorage-independent growth of breast cancer cells expressing a constitutively active TGFβ receptor I. Finally, apoptosis induced by etoposide increased in c-Myb-silenced TGFβ-treated ER+ cell lines. In summary, exposure of ER + breast cancer cells to TGFβ induces an increase of c-Myb expression, which is required for expression of EMT-associated markers, in vitro invasion and anchorage-independent growth. Furthermore, our findings suggest a potentially detrimental effect of TGFβ and c-Myb co-expression in breast cancer. © 2011 Landes Bioscience. |
Note | cited By 47 |
URL | https://www.scopus.com/inward/record.uri?eid=2-s2.0-82855170853&doi=10.4161%2fcc.10.23.18346&partnerID=40&md5=45c2877e85f54ebbc3cfb8e5a029bd79 |
DOI | 10.4161/cc.10.23.18346 |
Citation Key | Cesi20114149 |