For a comparison, EGFP SKBR3 cells alone were seeded and cell mor

For a comparison, EGFP SKBR3 cells alone were seeded and cell morphology was analyzed by fluorescent microscopy. Alternatively, quadrupli cates of 4104 tumor cells were seeded in MSC CM or culture medium in 96 well plates. Phase contrast images were taken in the IncuCyte ZOOM Kinetic Imaging System. Cell confluence was evaluated by IncuCyte ZOOM 2013A software based on the confluence masks www.selleckchem.com/products/ABT-888.html as recommended by manufacturer. Migration assay Fifty thousand EGFP SKBR3 per well were plated in trip licates in ImageLock 96 well plates and let to adhere for 16 hrs. Confluent monolayers were wounded with wound making tool, washed twice and supplemented with MSC CM or culture medium. As indicated, medium was supplemented with receptor tyrosine kinase inhibi tors 150 nM Pazopanib, 250 nM Sorafenib or 200 nM Sunitinib.

Images were taken every two hours for next 72 hrs in the IncuCyte ZOOM Kinetic Imaging System. Cell migration was evaluated by IncuCyte ZOOM 2013A software based on the relative wound density measurements and expressed as means of three inde pendent experiments run in triplicates SD. Gene expression analysis EGFP SKBR3 tumor cells were cultured with or without MSC CM for 6 days with everyday medium replenish ment. Total RNA was isolated from 5106 EGFP SKBR3 cultured with or without MSC CM. Cultured cells were collected by trypsinization, RNA isolated by NucleoSpin RNA II and treated with RNase free DNase. Total RNA was sub jected to control PCR to confirm the absence of genomic DNA contamination. RNA was reverse transcribed with RevertAid H minus First Strand cDNA Synthesis Kit.

200 ng of cDNA was ampli fied in standard PCR performed in 20 ul 1x PCR master mix with 0. 5 ul respective specific primers and DNase free water in DNA Engine Dyad Peltier Thermal Cycler with pre set amplification profile and horizontal electrophoresis was used for detection of amplicons. Each reaction was run with appropriate no template controls and negative control. Primer sequences were listed in Additional file 2. Quantitative PCR was performed in 1 ABsolute QPCR SYBR Green Mix, 0. 16 uM primers and 200 ng of template cDNA on Bio Rad CFX96 and analyzed by Bio Rad CFX Manager soft ware version 1. 6. Relative gene expression change was calculated according to Ct method. GAPDH and HPRT1 gene expression was taken as endogenous reference.

Analysis was performed twice in triplicates and data expressed as means SD. Multiplex and SDF 1 secretion analysis 5104 EGFP SKBR3, 2. 5104 AT MSCs alone, and 5104 SKBR3 cells mixed with 2. 5104 AT MSCs were plated in the wells of 24 well plates and cultured in 2 ml of complete culture medium for two days. Cell free supernatants were collected and subjected to human Bio Plex 27 plex Cytokine Assay. selleckbio Measurements were performed on Luminex 100 System in duplicates with two different AT MSCs isolates. Results were expressed as mean pg ml of culture medium SD.

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