首都医科大学学报
首都醫科大學學報
수도의과대학학보
JOURNAL OF CAPITAL UNIVERSITY OF MEDICAL SCIENCES
2015年
2期
276-281
,共6页
张露勇%罗菲亚%胡培丽%单纯%张淼
張露勇%囉菲亞%鬍培麗%單純%張淼
장로용%라비아%호배려%단순%장묘
胶质瘤%神经酰胺%自噬性死亡%JNK信号通路
膠質瘤%神經酰胺%自噬性死亡%JNK信號通路
효질류%신경선알%자서성사망%JNK신호통로
glioma cell%ceramide%autophagic cell death%JNK signaling pathway
目的:探讨神经酰胺对大鼠脑胶质瘤细胞C6自噬性死亡的影响及其作用机制。方法不同浓度神经酰胺作用于C6细胞后,用MTT法检测细胞的存活率,流式法检测细胞凋亡的改变;Western blotting及电镜的方法观察细胞自噬水平的改变,以及JNK及其下游靶分子c-Jun的磷酸化水平变化;最后进一步借助JNK特异性抑制剂SP600125抑制JNK的活性,观察其对神经酰胺诱导的细胞自噬情况的影响。结果与对照组相比,神经酰胺作用24 h后,C6细胞存活率明显降低,且具有剂量依赖性,差异有统计学意义(P<0.05);与对照组相比,神经酰胺作用24 h后,C6细胞死亡明显升高且具有剂量依赖性,差异有统计学意义(P<0.05),但其中凋亡性死亡比例较低;神经酰胺作用后细胞内自噬小体数目,LC3B/LC3A的比值,Beclin-1的表达水平,以及JNK和c-Jun磷酸化水平都显著升高,差异具有统计学意义(P<0.05);提前给予JNK特异性抑制剂SP600125抑制JNK的活性后,显著阻断神经酰胺诱导的细胞自噬。结论神经酰胺可诱导胶质瘤细胞C6发生自噬性死亡,其诱导胶质瘤细胞发生自噬的机制可能与激活JNK信号通路有关。
目的:探討神經酰胺對大鼠腦膠質瘤細胞C6自噬性死亡的影響及其作用機製。方法不同濃度神經酰胺作用于C6細胞後,用MTT法檢測細胞的存活率,流式法檢測細胞凋亡的改變;Western blotting及電鏡的方法觀察細胞自噬水平的改變,以及JNK及其下遊靶分子c-Jun的燐痠化水平變化;最後進一步藉助JNK特異性抑製劑SP600125抑製JNK的活性,觀察其對神經酰胺誘導的細胞自噬情況的影響。結果與對照組相比,神經酰胺作用24 h後,C6細胞存活率明顯降低,且具有劑量依賴性,差異有統計學意義(P<0.05);與對照組相比,神經酰胺作用24 h後,C6細胞死亡明顯升高且具有劑量依賴性,差異有統計學意義(P<0.05),但其中凋亡性死亡比例較低;神經酰胺作用後細胞內自噬小體數目,LC3B/LC3A的比值,Beclin-1的錶達水平,以及JNK和c-Jun燐痠化水平都顯著升高,差異具有統計學意義(P<0.05);提前給予JNK特異性抑製劑SP600125抑製JNK的活性後,顯著阻斷神經酰胺誘導的細胞自噬。結論神經酰胺可誘導膠質瘤細胞C6髮生自噬性死亡,其誘導膠質瘤細胞髮生自噬的機製可能與激活JNK信號通路有關。
목적:탐토신경선알대대서뇌효질류세포C6자서성사망적영향급기작용궤제。방법불동농도신경선알작용우C6세포후,용MTT법검측세포적존활솔,류식법검측세포조망적개변;Western blotting급전경적방법관찰세포자서수평적개변,이급JNK급기하유파분자c-Jun적린산화수평변화;최후진일보차조JNK특이성억제제SP600125억제JNK적활성,관찰기대신경선알유도적세포자서정황적영향。결과여대조조상비,신경선알작용24 h후,C6세포존활솔명현강저,차구유제량의뢰성,차이유통계학의의(P<0.05);여대조조상비,신경선알작용24 h후,C6세포사망명현승고차구유제량의뢰성,차이유통계학의의(P<0.05),단기중조망성사망비례교저;신경선알작용후세포내자서소체수목,LC3B/LC3A적비치,Beclin-1적표체수평,이급JNK화c-Jun린산화수평도현저승고,차이구유통계학의의(P<0.05);제전급여JNK특이성억제제SP600125억제JNK적활성후,현저조단신경선알유도적세포자서。결론신경선알가유도효질류세포C6발생자서성사망,기유도효질류세포발생자서적궤제가능여격활JNK신호통로유관。
Objective To observe the autophagy of glioma cell induced by ceramide and explore the possible mechanism. Methods The viability of C6 cells was measured by MTT assay. The cell apoptosis was assayed by flow cytometry. Autophagic-related protein expressions of LC3B/ LC3A and Beclin-1 were determined by Western blotting. The level of JNK-c-Jun induced by ceramide was measured by Western blotting with or without the treatment of JNK specific inhibitor SP600125. Results After treatment of ceramide for 24 hours, the growth of C6 cells were significantly inhibited in dose-dependent manner(P<0. 05); and ceramide increased autophagic cell death also in dose-dependent manner(P <0. 05). Compared with the control group, the levels of LC3B/ LC3A and Beclin-1 were significantly increased in ceramide treatment group(P<0. 05). JNK was activated in the C6 cells exposed to ceramide and the phosphorylation of c-Jun also increased. This activation of autophagy could be reversed by the pre-treatment of SP600125. Conclusion Ceramide may induce autophagy in glioma cell and the mechanism may be related to the activation of JNK-c-Jun signaling pathway.
