Supplementation of recombinant transforming growth factor beta (TGF-beta) enhanced the spheroid formation capacity of HCC cells, and this effect was abolished when cultured with neutralizing antibodies against TGF-beta. Co-injection of HCC cells with fibroblasts but not with stellate cells or endothelial cells resulted in
the high motility of mice with high frequency of lung metastasis. [Conclusions] Fibrotic liver microenvironment accelerates PD98059 the malignant natures of HCC with enrichment of EpCAM/CD1 33-positive cancer stem cells through activation of TGF-beta signaling. TGF-beta may be a good molecular target to reduce the risk of aggressive liver cancer development in liver cirrhosis patients. Disclosures: Mariko Yoshida – Grant/Research Support: Bayer Shuichi Kaneko – Grant/Research Support: MDS, Co., Inc, Chugai Pharma., Co., Inc, Toray Co., Inc, Daiichi Sankyo., Co., Inc, Dainippon Sumitomo, Co., Inc, Aji-nomoto Co., Inc, MDS, Co., Inc, Chugai Pharma., Co., Inc, Toray Co., Inc, Daiichi Sankyo., Co., Inc, Dainippon Sumitomo, Co., Inc, Ajinomoto Co., Inc, Bayer Japan The following people have nothing to disclose: Mitsumasa Kondo,
Taro Yamashita, Naoki Oishi, Kouki Nio, Sha Sha Zeng, Takehiro Hayashi, Yoshimoto Nomura, Tomoyuki Hayashi, Hikari Okada, Hajime Sunagozaka, Hajime Takatori, Honda Masao Background::The presence of liver cirrhosis is the main risk factor for the development of hepatocellular carcinoma (HCC). Activated hepatic stellate cells (aHSC) are recognized SCH772984 ic50 as a central event in the development of liver fibrosis, but which role in HCC is unclear. Objective:This study investigated angiogenetic activity of aHSC in HCC and angiogenetic effect on proliferation, metastasis of HCC. Methods:In vitro, we exposured microvascular endothelial cell (MEC) HAS1 to conditioned media(CM) from aHSC to observe the influence of the CM on MEC by quantifying MEC tube formation, and placed aHSC over an endothelial monolayer to assesse transendothelial migration of aHSC to hepatoma cells by examining the movement of CFSE labeled aHSC through the endothelial cell monolayer. For convenient viewing, aHSC were labeled
for CFSE (one green fluorescent dye). In vivo, we established orthotopic model of HCC with nude mice receiving an intraliver injection of aHSC plus hepatoma cells. After 7 weeks, tumor size,number of metas-tases were measured. Forthermore, tumors tissue were ashah-sessed by immunostaining for expression of aHSC and microvessel. Angiogenesis activities were assessed by immunostaining tumors for CD34, an endothelial cell marker and vascular endothelial growth factor (VEGF). Results: In vitro, The CM from aHSC stimulated the tube formation by MEC, and hepatoma cells stimulated transendothelial migration of aHSC. In vivo, compared with mice receiving hepatoma cells alone, mice injected with hepatoma cells plus aHSC exhibited the most increased tumor size and regional and distant metastasis.
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