印楝素对SL-1的细胞凋亡诱导作用

本文以喜树碱（camptothecin）作对比,以二甲基亚砜（DMSO）作对照,系统研究了印楝素（azadirachtin）对斜纹夜蛾Spodoptera litura离体细胞系（SL-1）的凋亡诱导作用。印楝素0.75μg/mL处理后SL-1细胞后12-72h,倒置显微镜观察可见大量细胞皱缩,体积变小,胞膜气泡化,与邻周细胞脱落,胞浆浓缩,胞膜突起,细胞器密集,核染色质浓缩并凝聚在核膜周边,出现大量凋亡小体;AO染色荧光显微镜观察可见细胞核内致密明亮黄绿色荧光和亮绿色或橘黄色的凋亡小体;透射电镜观察可见细胞皱缩、微绒毛消失、染色质浓缩和边缘化、核膜皱缩界限模糊、部分线粒体嵴结构消失和数量明显增加的吞噬泡等细胞凋亡典型形态学特征;TUNEL实验可见大量被标记为小圆形或环形黄绿色或绿色荧光的阳性凋亡细胞。流式细胞仪测定表明,印楝素0.75μg/mL处理后48h凋亡率最高达11.45%,比对照提高381.3倍;而喜树碱以1.72μg/mL处理亦对SL-1具有相似的诱导作用,处理后36h凋亡率最高达到17.42%。扫描电镜观察表明,印楝素和喜树碱处理后,SL-1细胞表面没有形成明显的“孔”、“洞”、“门”之类的结构破坏。推测印楝素与喜树碱对SL-1的凋亡信号转导方式和途径不同,导致细胞凋亡时序性不同。

植物源物质诱导的斜纹夜蛾细胞凋亡

为了研究植物源物质对斜纹夜蛾Spodoptera litura离体培养细胞系SL-1的凋亡诱导作用,采用倒置相差显微镜观察了印楝素、喜树碱等9种物质各自对SL-1凋亡小体的浓度效应及时序性。结果表明：印楝素0.1～5.0μg/mL和喜树碱0.5～20.0μmol/L处理SL-1,24～48h后均产生大量典型的凋亡小体;茶皂素、蓖麻碱、黄樟油、丹皮酚、烟碱、苦参碱和博落回碱0.1～20.0μg/mL处理SL-1后,整个观察期72h内均无明显凋亡小体出现,凋亡诱导作用不明显。印楝素0.75μg/mL诱导SL-1细胞凋亡,从凋亡小体判断,处理后0～36h属细胞凋亡早期,36～60h属细胞凋亡中期,60h后为细胞凋亡晚期。喜树碱5.0μmol/L诱导SL-1细胞凋亡,处理后0～24h属细胞凋亡前期,24～54h属细胞凋亡中期,54h后进入细胞凋亡晚期。初步认为印楝素和喜树碱对SL-1有凋亡诱导作用,并具有一定的浓度依赖性和时序性。

斜纹夜蛾铁硫亚基蛋白的表达及功能鉴定

铁硫亚基蛋白(rieske iron-sulfur protein,RISP)是线粒体复合物Ⅲ的关键蛋白亚基之一,在呼吸链电子传递过程中起到重要作用。本研究通过RT-PCR克隆得到斜纹夜蛾Spodoptera litura RISP基因SlitRISP的ORF,构建了pET32a-SlitRISP原核表达载体,SDS-PAGE和Western blot检测结果显示,SlitRISP原核表达蛋白以包涵体的形式存在于菌体沉淀中,且RISP抗体可成功用于该蛋白的免疫印迹检测。为了进一步鉴定SlitRISP在斜纹夜蛾离体细胞系SL-1中的功能,通过向细胞内转染siRNA,利用RNAi技术沉默SL-1中的SlitRISP。qRT-PCR结果表明,分别经50nmol/L和100nmol/L siRNA处理48h后,SL-1中SlitRISP的表达均几乎完全被抑制;Western blot结果显示,SL-1中SlitRISP含量显著低于CK。当SL-1SlitRISP被成功沉默后,通过检测SL-1线粒体膜电位、细胞ATP含量和细胞增殖抑制率鉴定RISP在线粒体电子传递过程中的重要作用。流式细胞仪测定结果表明,经50nmol/L和100nmol/LsiRNA处理24h后,SL-1线粒体膜电位相对于CK分别降低23.52%和11.32%,而处理48h后,SL-1线粒体膜电位则分别升高5.58%和27.66%;siRNA处理24h和48h后,SL-1ATP含量相对于CK分别降低82.71%和84.50%,最终导致SL-1细胞增殖抑制率分别为53.64%和67.94%。这些结果表明SlitRISP在SL-1中参与线粒体膜电位的形成和细胞ATP的合成。介于RISP在线粒体电子传递链中的重要作用,其可能成为新型杀虫作用靶标,这可为研制新型呼吸抑制剂提供参考。

斜纹夜蛾细胞的微载体悬浮培养

当微载体浓度３ｍｇ／ｍＬ、细胞接种浓度１．８０×１０５细胞／ｍＬ时，细胞培养８ｄ达最大生长密度１．２０×１０６细胞／ｍＬ，细胞群体倍增时间５６．２ｈ，葡萄糖的浓度随细胞培养时间的延续逐渐减小；氨的浓度随细胞培养时间的延续逐渐递增．

CSA对SfaMNPV诱导SL-1细胞凋亡的影响

检测线粒体膜通透性转运孔(MPT)的开放抑制剂环孢菌素A(CSA)对芹菜夜蛾核型多角体病毒(Syngrapha falcifera multiplenuclear polyhedrosis virus,SfaMNPV)诱导诱导斜纹夜蛾(Spodoptera litura Cells,SL-1)细胞凋亡的影响。用不同浓度CSA和SfaMNPV单独或联合处理SL-1细胞,通过细胞形态学观察、DNA凝胶电泳法、PI染色流式细胞仪鉴定细胞凋亡,应用罗丹明123(Rh123)染色流式细胞仪测定线粒体跨膜电位(ΔΨm)。CSA明显抑制了SfaMNPV诱导的SL-1细胞凋亡,CSA还抑制了SfaMNPV诱导的SL-1细胞线粒体膜电位(ΔΨm)下降。CSA抑制了SfaMNPV诱导SL-1细胞的ΔΨm下降,可能是亲环素-D(CyP-D)与CSA的结合导致MPT的关闭,从而抑制细胞凋亡。

Mitochondrial response and calcium ion change in apoptotic insect cells induced by SfaMNPV

Mitochondrial responses and changes of cal- cium ions in apoptotic insect SL-1 cells induced by Syn- grapha falcifera multiple nuclear polyhedrosis virus (SfaMNPV) are reported in this paper. By using Rhodamine 123 as a fluorescent labeling probe, flow cytometry analysis and confocal laser scanning microscope observation we observed that the mitochondrial transmembrane potential (?Ψm) began to decrease in SL-1 cells at 4 h post infection and ?Ψm reduced continuously with the extension of virus infection. Western blotting indicated that the Bcl-2 level in the mitochondria gradually declined and was down- regulated. Cells undergoing apoptosis were found to have an elevation of cytochrome c in the cytosol and a corresponding decrease in the mitochondria, which indicated that cytochrome c was released from mitochondria into cytosol. These results suggest that mitochondrion-mediated apoptotic signal transduction pathway exists in apoptotic insect cell induced by SfaMNPV. Cytosolic free calcium ([Ca2+]i) concentration rapidly increased after SfaMNPV infection and the elevated calcium was tested to come partly from extracelllular calcium ion influx. Flow cytometry analysis indicated that the apoptosis in SL-1 cells was not influenced by established cytosolic calcium clamped conditions and the EGTA inhibiting calcium influx. Therefore, neither the elevation of cytosolic calcium ion nor extracellular calcium entry was the inducing factor of apoptosis, which hinted that the depletion of ER Ca2+ store contributed to SL-1 cell apoptosis induced by SfaMNPV.