In the process of IT-inducd apoptosis, caspase-3 appeared to play a role. We investigated whether caspase-3 is regulated in anti-c-Met/PE38KDEL-induced cell death. As shown in Figure 6, procaspase-3 was proteolytically cleaved in a dose-dependent see more manner after 24 hr of IT treatment, resulting in the production of the active caspase-3 fragment (17 kDa). In untreated control cells (0 ng/ml), no caspase-3 was detected. All these results suggested that IT anti-c-Met/PE38KDEL causes apoptosis at least partially via activation of caspase-3. Figure 6 IT-induced caspase 3 cleavage. Lysates from normal gastric GSK461364 ic50 mucosa cells GES-1 and GC cell lines MKN-45

and SGC7901 with or without IT treatment were analyzed for procasoase-3 protein levels and activated caspase protein levels by western blot using an anti- procaspase-3, anti-activated caspase-3 and anti- β-actin antibodies (loading control). Discussion GC is the second leading cause of cancer mortality in the world [20]. The receptor tyrosine kinase c-Met is constitutively activated in many GCs [2]. Selleckchem Blebbistatin Amplifications of c-Met have been associated with human GC progression [21] C-Met is also related to lymph node metastasis in GC [22]. Therefore, c-Met is considered a promsing therapeutic target for this type of cancer [3]. The aim of this study was to evaluate the effects of recombinant immunotoxin anti-c-Met/PE38KDEL on proliferation

and apoptosis of GC cells and explore the mechanism underlying the action of anti-c-Met/PE38KDEL. SGC7901 was derived from moderately differentiated GC, with a high metastatic potential [23]. MKN-45 was derived from poorly differentiated GC with low metastatic potential [24]. We found that SGC7901 cells expressed high level of c-Met than MKN-45 cells. Normal gastric mucosa cells GES-1 expressed a minimum level of c-Met. Studies have shown that c-Met overexpression in carcinoma cells Amylase is associated with liver metastasis of GC [25]. Moreover; c-Met expression can be used as an

indicator of liver metastasis for GC patients. It has also been reported that HGF is a lymphangiogenic factor, which can directly or indirectly stimulate lymphangiogenesis and contribute to lymphatic metastasis in GC [26]. Therefore, we hypothesized that IT anti-c-Met/PE38KDEL may be effective in preventing GC’s metastasis. Our data showed that IT decreased GC cell proliferation in a time- and dose-dependent manner. After 48 hr of IT treatment (100 ng/ml), cell inhibition rate in MKN-45 and SGC7901 cells was about 75% and 95%, but only 30% in GES-1 cells, presumably due to low c-Met expression on GES-1 than the two GC cells. IT attenuates cancer cell growth not only by inhibiting protein synthesis but also by inducing apoptosis [27]. We found that IT anti-c-Met/PE38KDEL induced a rapid inhibition of protein synthesis with simultaneous induction of apoptosis in GC cells.