The transmembrane protein-tyrosine phosphatase (PTP) DEP-1 (density-enhanced phosphatase) is a candidate tumor suppressor in the colon epithelium. We have explored the function of DEP-1 in colon epithelial cells by inducible re-expression in a DEP-1-deficient human colon cancer cell line. Density-enhanced phosphatase-1 reexpression led to profound inhibition of cell proliferation and cell migration, and was associated with cytoskeletal rearrangements. These effects were dependent on the PTP activity of DEP-1 as they were not observed with cells expressing the catalytically inactive DEP-1 C1239S variant. shRNA-mediated suppression of DEP-1 in a colon epithelial cell line with high endogenous DEP-1 levels enhanced proliferation, further supporting the antiproliferative function of DEP-1. Nutrients, which are considered to be chemoprotective with respect to colon cancer development, including butyrate, green tea and apple polyphenols, had the capacity to elevate transcription of endogenous DEP-1 mRNA and expression of DEP-1 protein. Upregulation of DEP-1 expression, and in turn inhibition of cell growth and migration may present a previously unrecognized mechanism of chemoprevention by nutrients.Oncogene ( . The capacity of DEP-1 to antagonize signaling of these tyrosine kinases may relate to its antitransforming activity. Furthermore, the locus Scc-1, which has been linked with susceptibility to colon cancer in mice, harbors the PTPRJ gene (Ruivenkamp et al., 2002). Loss of heterozygosity for DEP-1 has previously been described in about 71% (25 of 35) cases of colon carcinoma and 47% (22 of 47) of colon adenoma samples (Ruivenkamp et al., 2003).Little is known about DEP-1 expression in colon carcinoma at the protein level. We therefore, analysed a panel of colon cell lines for DEP-1 protein expression. As shown in Figure 1a, expression in the analysed cell lines varies from relatively high levels in LT 97 adenoma cells and HT 29, DLD-1, HCT-16, COGA-1 and COGA-12 colon carcinoma cells, to relatively low levels in LOVO, Colo-320, COGA-2 and COGA-3 cells, and no detectable DEP-1 protein expression in SW 480 cells. To analyse the functional effects of DEP-1 expression, we chose the DEP-1-negative SW 480 cell line to reexpress the PTP. cDNA encoding wild-type human DEP-1, or the catalytically inactive DEP-1 C1239S was transferred into the bicistronic, tetracycline-regulated (tet-off) expression vector pNRTIS21 (Tenev et al., 2000). SW 480 cells were transfected with the corresponding constructs, and resistant cell clones were selected and screened for inducible DEP-1 expression. In selected cell clones, expression of DEP-1 wild-type or the DEP-1 CS mutant to comparable levels occurred in the absence of anhydrotetracylin (ATC), whereas only very low levels of DEP-1 protein were detectable in its presence (Figure 1b).These cell lines were analysed for biological effects of DEP-1 re-expression. Cell proliferation in presence of wild-type DEP-1 was clearly reduced as compared to cells with suppressed DEP-1 expression (Fig...
