Transient but Not Stable ZEB1 Knockdown Dramatically Inhibits Growth of Malignant Pleural Mesothelioma Cells

被引:5
|
作者
Horio, Mihoko [1 ]
Sato, Mitsuo [1 ]
Takeyama, Yoshihiro [1 ]
Elshazley, Momen [1 ]
Yamashita, Ryo [1 ]
Hase, Tetsunari [1 ]
Yoshida, Kenya [1 ]
Usami, Noriyasu [2 ]
Yokoi, Kohei [2 ]
Sekido, Yoshitaka [3 ,5 ]
Kondo, Masashi [1 ]
Toyokuni, Shinya [4 ]
Gazdar, Adi F. [6 ,7 ]
Minna, John D. [6 ,7 ]
Hasegawa, Yoshinori [1 ]
机构
[1] Nagoya Univ, Grad Sch Med, Dept Resp Med, Nagoya, Aichi 4648601, Japan
[2] Nagoya Univ, Grad Sch Med, Div Thorac Surg, Nagoya, Aichi 4648601, Japan
[3] Nagoya Univ, Grad Sch Med, Dept Canc Genet, Nagoya, Aichi 4648601, Japan
[4] Nagoya Univ, Grad Sch Med, Dept Pathol & Biol Responses, Nagoya, Aichi 4648601, Japan
[5] Aichi Canc Ctr, Res Inst, Div Mol Oncol, Nagoya, Aichi 464, Japan
[6] Univ Texas SW Med Ctr Dallas, Hamon Ctr Therapeut Oncol Res, Dallas, TX 75390 USA
[7] Univ Texas SW Med Ctr Dallas, Simmons Comprehens Canc Ctr, Dallas, TX 75390 USA
基金
日本学术振兴会;
关键词
LUNG-CANCER CELLS; TRANSCRIPTIONAL REPRESSOR; BREAST-CANCER; E-CADHERIN; ESTABLISHMENT; PROGRESSION; PHENOTYPE; POLARITY; THERAPY; MODEL;
D O I
10.1245/s10434-011-2142-0
中图分类号
R73 [肿瘤学];
学科分类号
100214 ;
摘要
Background. The role of ZEB1, a master epithelial-to-mesenchymal transition gene, in malignant pleural mesothelioma (MPM) is unclear. Methods. The expression of ZEB1, E-cadherin, vimentin, and epithelial cell adhesion molecule (EpCAM) in 18 MPM cell lines and a normal pleural mesothelial cell line MeT-5A was determined by quantitative real-time polymerase chain reaction and Western blot testing. RNA interference-mediated transient and/or stable knockdown of ZEB1 and EpCAM was performed. Microarray expression analysis was performed with a TORAY-3D gene chip. Growth was evaluated by colorimetric proliferation and colony formation assays. Luciferase reporter assay was performed to access the effects of ZEB1 knockdown on EpCAM promoter activity. Results. Most MPM cell lines exhibited mesenchymal phenotype and expressed ZEB1. Transient ZEB1 knockdown suppressed growth in all four cell lines studied (ACC-MESO-1, H2052, Y-MESO-8A, Y-MESO-29) while stable ZEB1 knockdown suppressed growth only in Y-MESO-29. Genome-wide gene expression analysis revealed that EpCAM was the most prominently up-regulated gene by both transient and stable ZEB1 knockdown in ACC-MESO-1, with more marked up-regulation in stable knockdown. We hypothesized that EpCAM up-regulation counteracts the stable ZEB1 knockdown-induced growth inhibition in ACC-MESO-1. Transient EpCAM knockdown suppressed growth dramatically in ACC-MESO-1 cells expressing shZEB1 but only modestly in those expressing shGFP, supporting our hypothesis. Luciferase reporter assay showed that ZEB1 knockdown resulted in increased EpCAM promoter activity. EpCAM was also up-regulated in Y-MESO-29 expressing shZEB1, but this EpCAM up-regulation did not counteract ZEB1knockdown-induced growth suppression, suggesting that the counteracting effects of EpCAM may be cellular context dependent. Conclusions. RNA interference-mediated ZEB1 knockdown may be a promising therapeutic strategy for MPM, but one has to consider the possibility of diminished growth inhibitory effects of long-term ZEB1 knockdown, possibly as a result of EpCAM up-regulation and/or other gene expression changes resulting from ZEB1 knockdown.
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页码:S634 / S645
页数:12
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