中华肝胆外科杂志
中華肝膽外科雜誌
중화간담외과잡지
CHINESE JOURNAL OF HEPATOBILIARY SURGERY
2009年
1期
45-48
,共4页
秦一雨%李济宇%李松岗%全志伟
秦一雨%李濟宇%李鬆崗%全誌偉
진일우%리제우%리송강%전지위
胆囊肿瘤%生长抑素%P53%Bax
膽囊腫瘤%生長抑素%P53%Bax
담낭종류%생장억소%P53%Bax
Gallbladder neoplasms%Somatostatin%P53%Bax
目的 通过前期实验发现,生长抑素(somatostatin,SST)作用于胆囊癌细胞株(GBC-SD)后,可显著增强阿霉素(doxorubicin,DOX)的杀伤能力[1].该实验旨在研究SST对GBC-SD细胞的诱导凋亡作用,并探讨其发生机制.方法 GBC-SD细胞分为4组:单独SST作用组、单独DoX作用组、联合用药组(SST预处理24 h后,再加入DOX)和对照组.药物作用24、36、48和60 h后,采用FITC-Annexin V/PI试验分别检测各组GBC-SD细胞的凋亡情况;另外运用Western印迹方法 检测SST作用24 h后,GBC-SD细胞内P53蛋白和Bax蛋白表达的变化.结果 SST分别作用24、36、48和60 h后,GBC-SD细胞没有出现明显的细胞凋亡,SST的致凋亡作用仅仅表现出微弱的时间依赖性;而在SST作用24 h后,GBC-SD细胞内的P53蛋白和Bax蛋白的表达都没有明显的变化(P>0.05).结论 SST不能诱导GBC-SD细胞产生明显的细胞凋亡,P53蛋白和Bax蛋白在其中发挥着重要作用.
目的 通過前期實驗髮現,生長抑素(somatostatin,SST)作用于膽囊癌細胞株(GBC-SD)後,可顯著增彊阿黴素(doxorubicin,DOX)的殺傷能力[1].該實驗旨在研究SST對GBC-SD細胞的誘導凋亡作用,併探討其髮生機製.方法 GBC-SD細胞分為4組:單獨SST作用組、單獨DoX作用組、聯閤用藥組(SST預處理24 h後,再加入DOX)和對照組.藥物作用24、36、48和60 h後,採用FITC-Annexin V/PI試驗分彆檢測各組GBC-SD細胞的凋亡情況;另外運用Western印跡方法 檢測SST作用24 h後,GBC-SD細胞內P53蛋白和Bax蛋白錶達的變化.結果 SST分彆作用24、36、48和60 h後,GBC-SD細胞沒有齣現明顯的細胞凋亡,SST的緻凋亡作用僅僅錶現齣微弱的時間依賴性;而在SST作用24 h後,GBC-SD細胞內的P53蛋白和Bax蛋白的錶達都沒有明顯的變化(P>0.05).結論 SST不能誘導GBC-SD細胞產生明顯的細胞凋亡,P53蛋白和Bax蛋白在其中髮揮著重要作用.
목적 통과전기실험발현,생장억소(somatostatin,SST)작용우담낭암세포주(GBC-SD)후,가현저증강아매소(doxorubicin,DOX)적살상능력[1].해실험지재연구SST대GBC-SD세포적유도조망작용,병탐토기발생궤제.방법 GBC-SD세포분위4조:단독SST작용조、단독DoX작용조、연합용약조(SST예처리24 h후,재가입DOX)화대조조.약물작용24、36、48화60 h후,채용FITC-Annexin V/PI시험분별검측각조GBC-SD세포적조망정황;령외운용Western인적방법 검측SST작용24 h후,GBC-SD세포내P53단백화Bax단백표체적변화.결과 SST분별작용24、36、48화60 h후,GBC-SD세포몰유출현명현적세포조망,SST적치조망작용부부표현출미약적시간의뢰성;이재SST작용24 h후,GBC-SD세포내적P53단백화Bax단백적표체도몰유명현적변화(P>0.05).결론 SST불능유도GBC-SD세포산생명현적세포조망,P53단백화Bax단백재기중발휘착중요작용.
Objective In the previous research, after the treatment of somatostatin, the lethal effects of doxorubicin on gallbladder carcinoma were significantly enhanced. To identify the cytotoxici-ty of SST on GBC-SD cells, apoptosis index of GBC-SD cells after treatment of somatostatin or doxo-rubicin or co-use of somatostatin and doxorubicin was observed. Methods GBC-SD cells were divided into four groups: SST-alone-treated group, DOX-alone-treated group, co-treated group (co-treatment of SST and DOX) and the control group. In control group, the cells were cultivated by medium only. In SST-alone-treated group, the cells were cultivated by medium with SST in the concentration of 75 μg/ml. In DOX-alone-treated group, the cells were cultivated by medium with DOX in the concentra-tion of 5 μg/ml. In the co-treated group, cells were firstly cultivated by medium with 75 μg/ml SST for 24 h, followed by the addition of DOX in the concentration mentioned above. After treatment of the GBC-SD cells, apoptotic index was determined by FITC-Annexin V/PI assay at 24, 36, 48 and 60 h, respectively. Twenty-four hours after the treatment of SST, the expressions of P53 and Bax in GBC-SD cells was examined by western blot. Results After treatment of SST, no significant cell ap-optosis occurred. Only a weak time-dependent cytotoxicity of SST was observed. And 24 h after treat-ment of SST, the expression of P53 and Bax did not significantly varied either. Conclusion SST can not induce significant apoptosis of GBC-SD cells, in which P53 and Bax may play a critic role.
