To determine no matter if ubiquitinproteasome pathway is involved in rebamipide action on survivin expression degree, AGS cells have been pretreated with proteasome inhibitor, MG-132, 10 lM, 30 min before therapy with either medium or rebamipide 5 mg/ml for 6 h. mRNA expression of survivin by RT/PCR. Human survivin unique RT-PCR primers employed for analysis of survivin mRNA expression by RT/PCR were purchased from R&D System . Cells had been directly lysed in Trizol Reagent for a RNA isolation. Total RNA from each sample was made use of in the reverse transcription reaction to synthesize first strand cDNA. Ten microliters of cDNA was put to use in each PCR. Western blot evaluation. Cell lysates containing equal amount of proteins have been subjected to SDS?PAGE and transferred onto a nitrocellulose membrane. The membrane was incubated with a precise, primary polyclonal survivin antibody followed by peroxidase-conjugated secondary antibody. Immunoreactive proteins have been visualized using ECL detection system .
Where indicated, the membrane was stripped and reprobed with another certain primary antibody. Protein signals had been quantified using Metamorph Imaging System, version 3.0 . Indicated protein signal intensities from the Western blots were subtracted from background signal intensities. Immunohistochemistry. AGS cells were plated on coverslips and grown to _70% confluence. Cells were subjected chemical screening to various treatments as indicated, fixed with 4% paraformaldehyde for 20 min at room temperature, then with cold acetone for five min, and blocked with Superblock for 7 min at room temperature. After washing with PBS, coverslips had been incubated with antisurvivin or anti-Aurora-B antibodies for 2 h at room temperature. After washing with PBS, coverslips have been incubated with secondary antibodies: anti-rabbit Texas Red-conjugated for survivin and anti-mouse FITC-conjugated for Aurora-B for 40 min at room temperature.
Coverslips had been then mounted and images have been captured using a Nikon digital camera DXM1200 attached to a Nikon Optiphot fluorescence microscope. Survivin mRNA and protein are strongly expressed in gastric cancer AGS cells as reflected by RT/PCR , Western blotting , and immunostaining price WHI-P 154 . Immunostaining demonstrated expression of survivin in _52% of cancer cells, strong staining predominantly localized to the nuclei . Aurora-B is also strongly expressed in AGS cells, often co-expressed and co-localized with survivin, especially in the mitotic spindle of cells undergoing divisions . Treatment with specified survivin siRNA significantly knock down survivin expression and significantly reduced cell viability .
Treatment with rebamipide significantly reduced survivin mRNA and protein expression and reduced Aurora-B and cell proliferation . Pretreatment with the proteasome inhibitor, MG-132, did not affect rebamipide-induced downregulation of survivin in AGS cells , indicating that ubiquitin? proteasome pathway is not involved in the mechanism of rebamipide action on survivin in AGS cells.