After 24-hour incubation in DMEM with FCS, the culture medium wa

After 24-hour incubation in DMEM with FCS, the culture medium was changed to serum-free DMEM, and all experiments were performed 24 hours later. This purification procedure has well been established [11, 12], and >95% of the cells obtained by this method were cardiomyocytes. 2.2. Plasmid DNA Preparation of rat hepatocyte growth factor (HGF) expression plasmid Inhibitors,research,lifescience,medical DNA was described previously [13]. Briefly, rat HGF cDNA cloned by polymerase chain reaction was inserted into the unique Xho I site between the cytomegalovirus immediate-early enhancer-chicken β-actin hybrid promoter and rabbit β-globin poly A site of the

pCAGGS expression plasmid [14]. The resulting plasmid, pCAGGS-HGF, was grown in Escherichia coli DH5α (Figure 1(a)). The plasmid was find more purified with a QUIAGEN plasmid Inhibitors,research,lifescience,medical DNA kit and dissolved in TE buffer. The purified plasmid DNA was stored at −20°C and diluted to the required concentration with distilled water immediately before use. Figure 1 (a) Structure of the expression plasmid

pCAGGS-HGF. The expression cassette of pCAGGS-HGF contains chicken β-actin promoter, rat HGF, and rabbit β-globin poly A. (b) Experimental setup. The transducer was attached to the bottom of the … 2.3. Bubble Liposome Inhibitors,research,lifescience,medical Liposome microbubble, SHU 508A, consists of palmitic acid and galactose and provides echogenic micron-sized air Inhibitors,research,lifescience,medical bubbles

when suspended in water. The diameter of bubbles ranges from 2 to 8μm, and 97% are smaller than 6μm [15]. These air bubbles are stabilized by palmitic acid, which forms a molecular film that lowers the surface tension of the aqueous vehicle. The SHU 508A bubbles are nontoxic, have a neutral pH, are biodegradable, and are made from a physiologically occurring substance. The physiochemical properties of SHU 508A bubbles are typical of a saccharide solution [15]. 2.4. Experiment on Ultrasound Mode Before performing the experiments Inhibitors,research,lifescience,medical for dose-effect relationships using liposome sonoporation, we needed to determine the most appropriate ultrasound mode for the sonoporation the procedure for efficient transfection. We tested four modes of ultrasound: pulsed wave Doppler, color flow Doppler, continuous wave Doppler, and harmonic power Doppler, which are available with standard echocardiographic machinery in a clinical laboratory. We performed a simple transfection experiment at the same acoustic pressure of 0.5W/cm² for each ultrasound mode, using a single condition with 60μg HGF plasmid DNA, 1 × 107particles/mL of SHU 508A liposome, 30sec insonification, 15min of DNA incubation, and 3 repetitions of insonification. Rat neonatal cardiomyocytes were inoculated and grown to confluence in DMEM+10% FCS.

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