Relative quantification was done using Ct measurements original site on SYBR Green based fluores cence readings with HPRT as a housekeeping gene. Mea surements were done in triplicate. Flow cytometry Protein expression of receptors on the tumor cell sur face was determined by flow cytometry. Cells were harvested using Accutase solution after 24 hours of normoxia, hypoxia and hyp oxia with bevacizumab treatment. Cells were labeled for Neuropilin1 with CD304 and VEGFR2 with CD309 APC conjugated antibodies and measured by a BD FACS Canto II flow cytometer. HUVEC were used Inhibitors,Modulators,Libraries as a control. Analysis was done using FlowJo software to determine the percentages of positive cells. Results represent averaged percentages from two biological repetitions. Propidium iodide stained cells were prepared by fixing the cells in 80% ice cold ethanol for up to 48 hours.
Cells were then washed with PBS and resuspended and incubated for 30 minutes in 38 mM sodium citrate, 24 ug ml RNase A and 54 uM propidium iodide prior to FACS measurement. Statistical analysis Unpaired, two tailed Students Inhibitors,Modulators,Libraries t test was performed for statistical analysis. A p value of 0. 05 was considered Inhibitors,Modulators,Libraries to indicate a significant difference. Results Cell line selection As VEGFA is thought to work primarily through activa tion of one of the known VEGF receptors VEGFR1, VEGFR2 and co receptor Neuropilin1, in general two Inhibitors,Modulators,Libraries cell lines per tumor type were selected from the NCI 60 panel of solid tumors, according to high relative expres sion levels from publicly available microarray data, published data and our own preliminary gene expression data related to angiogenesis pathway genes.
These cell lines are also representative of most of the indications where bevacizumab is approved for clinical use and has shown variable efficacy in clinical practice. Tumor cell expression of VEGF receptors The protein levels of VEGFR1, VEGFR2 and Neuropilin1 expressed by tumor cells were determined by western blot analysis. Inhibitors,Modulators,Libraries Total cell lysates from cells treated with or without bevacizumab under hypoxic conditions for 24 hours were examined to determine if there is any regu lation of receptor expression compared to normoxic con ditions. The two VEGFR2 specific bands were detected on HUVECs, which was used as a positive con trol and present in four of the selected tumor cell lines, H522, HOP62, HCT 116 and MDA MB 231.
Changes in expression of VEGFR2 as re sult of hypoxia or bevacizumab treatment in tumor cells were difficult to evaluate by western blot, so we there fore assessed transcript changes and localization by flow cytometry. VEGFR1 selleck inhibitor showed clear expression shown by two bands in all cell lines with the exception of H522. Whilst hypoxia up regulated expression in A498 by 1. 8 fold, bevacizumab treatment does not appear to strongly regulate VEGFR1 in the other VEGFR1 expressing cell lines.