超声介导HT29结直肠癌细胞体外转染的初步结果

R. Hart, L. Newman
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摘要

从一个不灭细胞系中提取HT29人结直肠癌细胞,用60mm培养皿在4个11mm的最小基本培养基上培养融合。一个盘子作为对照。用无血清培养基洗涤后,将1mg异硫氰酸荧光素(FITC)与牛血清白蛋白(BSA)结合,加入其余三个培养皿中。在培养皿2中加入FITC-BSA。在培养皿3和4中加入无菌充气微球(平均直径3 /spl mu/m),每个细胞约230个微球。用2.5 MHz脉冲波诊断谱多普勒超声无菌超声5分钟。然后将所有培养物在最低限度的基本培养基中继续培养24小时。随后用甲醇洗涤和干燥,用DPX培养基贴装,显微镜下观察。培养皿1、2和3显示出低水平的背景荧光,而培养皿4显示出强烈的细胞荧光。微球的存在促进了一种大分子(FITC偶联的BSA)进入HT29结直肠癌细胞的非致命性。
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Ultrasound mediated transfection of HT29 colorectal cancer cells in vitro: preliminary results
HT29 human colorectal cancer cells, from an immortal cell line, were grown to confluence on four 11 mm coverslips in minimal essential culture medium using 60 mm culture dishes. One dish was kept as a control. Following washing with serum-free medium, 1 mg of fluorescein isothiocyanate (FITC) conjugated with bovine serum albumin (BSA) was added to the remaining three dishes. FITC-BSA was added to dish 2. Sterile gas-filled microspheres (average diameter 3 /spl mu/m) were added to dishes 3 and 4, in an approximate ratio of 230 microspheres to each cell. Dish 4 was aseptically insonated using 2.5 MHz pulsed wave diagnostic spectral Doppler ultrasound for 5 minutes. All cultures were then on-grown for a further 24 hours in minimal essential culture medium. Subsequently they were washed and dried with methanol, mounted using DPX medium and microscopically viewed. Dishes one, two and three showed low levels of background fluorescence, while dish four showed strong cellular fluorescence. The presence of microspheres during insonation facilitates the non-lethal entry of a large molecule (FITC conjugated BSA) into HT29 colorectal cancer cells.
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