Statistical significance was declared if P < 0.05. Semiquantitative RT-PCR and real-time qPCR methods were used to compare EIF5A2 messenger RNA (mRNA) expression between 81 pairs of primary HCC tumor and nontumorous
surrounding tissues. Overexpression of EIF5A2 was detected in 50/81 (61.7%, P < 0.0001, independent Student's t test) of HCCs as compared to their nontumorous counterparts (Fig. 1A,B), indicating that EIF5A2 was frequently overexpressed in HCC. Among these 81 HCCs, detailed clinicopathological information was available for 45 cases. The association study found that CHIR-99021 cost overexpression of EIF5A2 was positively associated with tumor metastasis (P = 0.036, chi-square test) and negatively associated with tumor encapsulation formation (P = 0.020, chi-square test, Table 1), suggesting that EIF5A2 may play a role in HCC metastasis. Western blot analysis was applied to determine protein expression level of EIF5A2 in 12 cell lines including three immortalized liver cell lines (MIHA, LO2, and Chang Liver) and nine HCC cell lines (H2P, H2M, HepG2, Hep3B, Huh7, BEL7402, QSG7701, QGY7703, and PLC8024). EIF5A2 was undetectable in all three immortalized liver cell lines, whereas high-level expression of EIF5A2 was observed in 6/9 of HCC cell lines, including H2P, H2M, Hep3B, Huh7, BEL7402, and PLC8024
(Fig. 1C). The expression level of EIF5A in these 12 cell lines was also examined and a similar level of expression was observed in all tested cell lines, suggesting that EIF5A2, rather than EIF5A, www.selleckchem.com/products/MK-2206.html plays an oncogenic role in HCC development and progression. To investigate the role of EIF5A2 in HCC invasion and metastasis, EIF5A2 expression was compared between primary and metastatic HCCs by immunohistochemistry using an HCC tissue microarray containing 47 pairs selleckchem of HCC specimens. Each pair consisted of primary and metastatic
lesions derived from the same patient. In all, 25 pairs of HCCs (53.2%) showed higher expression of EIF5A2 in metastatic lesions compared with their individually matched primary tumor samples. In a subset of primary tumors, EIF5A2 protein expression was already elevated (18/47, 38.3%). IHC staining of EIF5A2 protein in representative samples of nontumor, primary, and metastatic lesions are shown in Fig. 1D. Moreover, in some metastatic lesions we observed that the expression level of EIF5A2 was obviously higher at the edge of tumor (Fig. 1E) and in tumor cells invading the surrounding tissue (Fig. 1F, indicated by arrows). We have described LO2-EIF5A2, a stable liver cell line overexpressing EIF5A2.11 Overexpression of EIF5A2 in LO2-EIF5A2 cells was determined by RT-PCR and western blot (Fig. 2A). Because cell motility is an important factor regulating cancer invasion and metastasis, the effect of EIF5A2 on cell motility was characterized by wound-healing, transwell migration, and Matrigel invasion assays.