中华实验外科杂志
中華實驗外科雜誌
중화실험외과잡지
CHINESE JOURNAL OF EXPERIMENTAL SURGERY
2014年
2期
333-335
,共3页
党丽峰%赵松%杨洋%刘东雷%吴恺%温丰标
黨麗峰%趙鬆%楊洋%劉東雷%吳愷%溫豐標
당려봉%조송%양양%류동뢰%오개%온봉표
超声微泡%食管癌%胞嘧啶脱氨酶:尿嘧啶磷酸核糖转移酶/5-氟胞嘧啶%基因治疗
超聲微泡%食管癌%胞嘧啶脫氨酶:尿嘧啶燐痠覈糖轉移酶/5-氟胞嘧啶%基因治療
초성미포%식관암%포밀정탈안매:뇨밀정린산핵당전이매/5-불포밀정%기인치료
Ultrasound microbubble%Esophageal cancer%Cytosine deaminsae : uracil phosphoribosyltransferase/5-flurocytosine%Gene therapy
目的 观察超声微泡(UM)介导的胞嘧啶脱氨酶:尿嘧啶磷酸核糖转移酶/5-氟胞嘧啶(CD:UPRT/5-FC)自杀基因系统对人食管癌细胞株EC9706的转染效率和对细胞活力的影响.方法 将EC9706细胞按1×108/L接种于12孔孔板中,随机分为4组:A组:空白对照组;B组:单纯质粒组;C组:单纯超声微泡组;D组:超声微泡+质粒组.24 h后在荧光显微镜下观察各组细胞绿色荧光蛋白的表达,流式细胞术(FCM)检测各组的转染效率,Western blot法检测各组细胞CD基因的表达,细胞计数试剂盒(CCK-8)法检测5-氟胞嘧啶(5-FC)对转染后细胞的杀伤作用.结果 (1)D组细胞中的绿色荧光强度明显高于其他各组,FCM检测各组转染成功率分别为0%、1.42%、0%、32.60%,超声微泡介导的转染对EC9706细胞活性无明显影响(P>0.05);(2)Western blot结果显示D组细胞CD基因蛋白条带灰度值明显高于其他各组(P<0.05);(3)5-FC对转染后的肿瘤细胞有明显的杀伤作用,细胞存活率明显下降.结论 采用超声微泡携带CD:UPRT融合自杀基因可显著提高在食管癌细胞中的转染效率,增强5-FC对肿瘤细胞的杀伤作用.
目的 觀察超聲微泡(UM)介導的胞嘧啶脫氨酶:尿嘧啶燐痠覈糖轉移酶/5-氟胞嘧啶(CD:UPRT/5-FC)自殺基因繫統對人食管癌細胞株EC9706的轉染效率和對細胞活力的影響.方法 將EC9706細胞按1×108/L接種于12孔孔闆中,隨機分為4組:A組:空白對照組;B組:單純質粒組;C組:單純超聲微泡組;D組:超聲微泡+質粒組.24 h後在熒光顯微鏡下觀察各組細胞綠色熒光蛋白的錶達,流式細胞術(FCM)檢測各組的轉染效率,Western blot法檢測各組細胞CD基因的錶達,細胞計數試劑盒(CCK-8)法檢測5-氟胞嘧啶(5-FC)對轉染後細胞的殺傷作用.結果 (1)D組細胞中的綠色熒光彊度明顯高于其他各組,FCM檢測各組轉染成功率分彆為0%、1.42%、0%、32.60%,超聲微泡介導的轉染對EC9706細胞活性無明顯影響(P>0.05);(2)Western blot結果顯示D組細胞CD基因蛋白條帶灰度值明顯高于其他各組(P<0.05);(3)5-FC對轉染後的腫瘤細胞有明顯的殺傷作用,細胞存活率明顯下降.結論 採用超聲微泡攜帶CD:UPRT融閤自殺基因可顯著提高在食管癌細胞中的轉染效率,增彊5-FC對腫瘤細胞的殺傷作用.
목적 관찰초성미포(UM)개도적포밀정탈안매:뇨밀정린산핵당전이매/5-불포밀정(CD:UPRT/5-FC)자살기인계통대인식관암세포주EC9706적전염효솔화대세포활력적영향.방법 장EC9706세포안1×108/L접충우12공공판중,수궤분위4조:A조:공백대조조;B조:단순질립조;C조:단순초성미포조;D조:초성미포+질립조.24 h후재형광현미경하관찰각조세포록색형광단백적표체,류식세포술(FCM)검측각조적전염효솔,Western blot법검측각조세포CD기인적표체,세포계수시제합(CCK-8)법검측5-불포밀정(5-FC)대전염후세포적살상작용.결과 (1)D조세포중적록색형광강도명현고우기타각조,FCM검측각조전염성공솔분별위0%、1.42%、0%、32.60%,초성미포개도적전염대EC9706세포활성무명현영향(P>0.05);(2)Western blot결과현시D조세포CD기인단백조대회도치명현고우기타각조(P<0.05);(3)5-FC대전염후적종류세포유명현적살상작용,세포존활솔명현하강.결론 채용초성미포휴대CD:UPRT융합자살기인가현저제고재식관암세포중적전염효솔,증강5-FC대종류세포적살상작용.
Objective To explore the transfection efficiency of cytosine deaminsae:uracil phosphoribosyltransferase/5-flurocytosine (CD:UPRT/5-FC) suicide gene system mediated by ultrasound microbubble (UM) for esophageal cancer in vitro,and indentify the effects on the cell viability.Methods EC9706 cells(l × 108/L) were seeded in the 12-well plates,and randomly divided into 4 groups:A.blank control group; B.CD:UPRT gene only; C.UM only; D.CD:UPRT gene and UM.After transfection,the expression of green fluorescent protein (gfp) was observed under the fluorescent microscopy and quantified by flow cytometry.Western blotting was used to detect the expression of CD protein.Different concentrations (0-160 mg/L) of 5-FC were added into the culture medium,then cells were cultured for another 36 h.The viability of EC9706 cells was measured by CCK-8 assay.Results (1) Gene fluorescence intensity and tansfection efficiency in group D were higher than other groups.The gene transfection efficiency in groups A,B,C,D and E was 0%,1.42%,0% and 32.60% respectively.The cell viability had no significant difference among groups before addition of 5-FC ; (2) CD protein in group D was higher than other groups (P < 0.05).(3) 5-FC had strong antitumor effect on successfully transfected esophageal cancer cells,almost all EC9706 cells in group D were killed when the concentration of 5-FC was above 80 mg/L.Conclusion Ultrasound microbubble can enhance the efficiency of gene transfection without obvious damage to cell viability in EC9706 cells.The method can also enhance the killing effect of CD:UPRT/5-FC suicide gene system in vitro.
