The fluorescence dye SYBR Green I intercalates with free siRNAs,

The fluorescence dye SYBR Green I intercalates with free siRNAs, resulting in a 22-bp fluorescent band under gel electrophoresis. Binding of PEI-NH-CNTs to siRNAs resulted in reduced availability of siRNAs for SYBR Green I intercalation, thus reducing the fluorescence signal [18, 20, 21, 28]. As shown in Figure 8, there was a gradual decrease in fluorescence intensity with increasing PEI-NH-CNT/PLX-4720 research buy siGAPDH mass ratios. The migration of siGAPDH was completely inhibited when the mass ratios of PEI-NH-SWNTs to siGAPDH and PEI-NH-MWNTs to siGAPDH were 80:1 and 160:1, respectively (Figure 8). These results indicate that both PEI-NH-SWNTs and PEI-NH-MWNTs could bind and form a stable

complex with siRNAs. Figure 8 Binding capacity of PEI-NH-SWNTs and PEI-NH-MWNTs towards siRNAs. PEI-NH-SWNTs (upper panel) and PEI-NH-MWNTs (lower panel) were complexed with a commercially available positive control siRNA against the selleck chemicals housekeeping gene glyceraldehyde 3-phosphate dehydrogenase (siGAPDH) at various www.selleckchem.com/products/gkt137831.html mass ratios, followed by EMSA. Cytotoxicity of PEI-NH-CNTs Human cervical cancer cells HeLa-S3 were treated with various concentrations of PEI-NH-SWNTs or PEI-NH-MWNTs for 48 h to examine their cytotoxicity. Viability of HeLa-S3

cells decreased with increasing concentrations of PEI-NH-CNTs (Figure 9). The half-maximal inhibitory concentrations (IC50) of PEI-NH-SWNTs and PEI-NH-MWNTs were 23.6 and 40.5 μg/ml, respectively. On the other hand, pure PEI was relatively toxic, with an IC50 of 0.56 μg/ml. At a concentration of 5 μg/ml, less than 2% of cells were viable in the presence of PEI, while 70% to 80% of cells were viable when incubated with PEI-NH-SWNTs or PEI-NH-MWNTs (Figure 9). These results suggest that PEI-NH-CNTs were less cytotoxic to HeLa-S3

cells compared to PEI. Figure 9 Cytotoxicity of PEI-NH-SWNTs and PEI-NH-MWNTs compared to PEI. Human cervical cancer cells HeLa-S3 were treated with 0 to 100 μg/ml of PEI-NH-SWNTs, PEI-NH-MWNTs, or pure PEI for 48 h. Cell viability was determined by MTT assay and expressed as the percentage of the optical density at 570 nm of treated cells relative to control cells. Error bars represent standard Unoprostone deviations (n ≥ 3). Statistical significance was observed at all concentrations of PEI-NH-SWNTs, PEI-NH-MWNTs, or pure PEI compared to the control (0 μg/ml). Transfection of siRNAs by PEI-NH-CNTs PEI-NH-CNTs were complexed with siGAPDH at mass ratios of 1:1, 10:1, and 20:1 and incubated with HeLa-S3 cells to achieve a final siGAPDH concentration of 30 nM. After 48 h, transfection efficiency of PEI-NH-CNTs was evaluated by the mRNA level of GAPDH and was compared with that of DharmaFECT. Transfection of siGAPDH with DharmaFECT resulted in more than 50% suppression of the mRNA level of GAPDH (Figure 10). Delivery of siGAPDH by PEI-NH-SWNTs suppressed GAPDH mRNA expression to 18%, 50%, and 62% of untreated control at PEI-NH-SWNT/siGAPDH ratios of 1:1, 10:1, and 20:1, respectively.

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