Smac/DIABLO在过氧化氢所致C2C12肌原细胞凋亡中的作用

为探讨Smac/DIABLO在过氧化氢(H₂O₂）所致C₂C₁₂肌原细胞凋亡中的作用,采用Hoechst 33258染色,观察H₂O₂ (0.5 mmol/L)处理C₂C₁₂肌原细胞不同时间后,细胞核形态学改变并计算凋亡核百分率,DNA抽提及琼脂糖电泳观察凋亡特征性梯状带,利用细胞成分分离后蛋白质印迹分析H₂O₂是否导致Smac/DIABLO从线粒体释放,采用Caspase检测试剂盒及蛋白质印迹分析Caspase-3和Caspase-9的活化,转染Smac/DIABLO基因,观察Smac/DIABLO过表达对H₂O₂所致的C₂C₁₂肌原细胞凋亡的影响.结果表明:H₂O₂处理1 h后,Smac/DIABLO从C₂C₁₂肌原细胞线粒体释放入胞浆,2 h更明显;H₂O₂处理4 h后,Caspase-3和Caspase-9活化,12 h达高峰;H₂O₂处理24 h后,C₂C₁₂肌原细胞显示特征性的凋亡形态改变,凋亡核百分率明显升高,DNA电泳出现明显“梯状”条带.与单纯过氧化氢损伤组相比,Smac/DIABLO高表达的C₂C₁₂肌原细胞经过氧化氢损伤组的Caspase-3和Caspase-9的活化、凋亡核百分率的升高、“梯状”条带的出现均更明显.结果表明,H₂O₂可导致Smac/DIABLO从C₂C₁₂肌原细胞线粒体释放,促进Caspase-9和Caspase-3的活化而促进细胞凋亡的发生.     

测定线粒体细胞色素c,c1,b,aa3含量的简单方法

线粒体是细胞中的重要细胞器,能量代谢的主要场所.在呼吸链中,细胞色素c,c_1,b,aa_3起着电子传递中间体的作用,其任何一种含量的减少或缺失将影响细胞的呼吸功能.由于细胞色素是一类带有卟啉环的蛋白质,在可见光区域有明显的吸收,可以利用这一性质进行比色定量。J.N.Williams首先建立了测定线粒体还原-氧化差光谱计算细胞色素含量的方     

邻二氮菲－Fe2＋氧化法检测H2O2／Fe2＋产生的羟自由基

报告检测H₂O₂/Fe^2＋所产生羟自由基的新方法. 羟自由基氧化反应后, 邻二氮菲-Fe^2＋的A₅₃₆明显下降, 且△A₅₃₆与邻二氮菲, FeSO₄及H₂O₂呈量效关系, 随反应时间延长, △A₅₃₆依幂函数规律上升. 此法试验结果表明, 甘露醇, 抗坏血酸及硫肥清除羟自由基作用呈明显的量效关系.     

香菇C91-3转录本Unigene 24277基因克隆表达及其生物学活性的研究

通过对香菇C_91-3转录本Unigene 24277基因的生物信息学分析,克隆表达含RCC1结构域的Unigene 24277基因,并研究其抗肿瘤活性。从香菇C_91-3菌丝体中提取总RNA,反转录合成cDNA,并利用Rapid Amplification of cDNA Ends（RACE）技术获得基因全长。NCBI数据库分析提示其含有RCC1结构域。PCR扩增RCC1结构域,将其克隆产物与pET-32a（+）载体连接,热转化至E.coil Rosetta-gami（DE3）中诱导表达,纯化、复性后,通过MTT法研究其抗肿瘤活性。结果显示原核表达载体构建成功,重组蛋白成功诱导表达,并初步证明了重组蛋白具有抑制肿瘤细胞增殖活性的功能,为后续抗肿瘤机制的探究奠定了基础。     

C3和C4植物寄主对华北地区棉铃虫越冬代和第一代的影响

确定华北越冬代棉铃虫虫源及其对第一代棉铃虫种群的影响是制定棉铃虫防治策略的基础。以越冬代棉铃虫蛾翅的稳定同位素δ¹³C为天然标记直接判定这些成虫的幼虫期寄主类型,并将雌虫接到春小麦植株上,调查其产卵、孵化、幼虫发育至化蛹、羽化等特征。结果表明,越冬代来自C₃植物(主要为棉花)的成虫个体数量占全部越冬羽化种群的53.1%,所产生的下一代老熟幼虫也较C₄来源的多(55.1%);雌蛾受精率都比较高;卵孵化率较高(52.9%>41.6%);幼虫发育在低龄阶段较比后者快,存活率低,但在高龄幼虫阶段相对后者慢,存活率高;与C₄植物(主要玉米)的来源个体后代的幼虫发育总历期接近,总存活率也相近。显示寄主植物小麦提供的营养条件在第一代棉铃虫的幼虫发育中具有决定性意义,即小麦只在特定阶段才适合幼虫的发育;而且不论是C₃还是C₄寄主来源的越冬代棉铃虫已经适应了这一限制。有效地评价了玉米和棉花等寄主植物对华北地区越冬代和次年第一代棉铃虫的影响,对于分析越冬代棉铃虫的虫源性质和第一代棉铃虫的防治及Bt抗性的治理有重要参考价值。     

血红蛋白A2现象发生机制的研究——“红细胞HbA2”为HbA2与HbA的结合产物

为了弄清血红蛋白A₂现象的发生机制,我们对“红细胞HbA₂”的化学组成进行了分析。“红细胞HbA₂”的双向电泳结果表明,它含有两种血红蛋白成分:一种相当于HbA,另一种很可能是溶血液HbA₂。其单向二次电泳结果也证明,它是由溶血液HbA₂和HbA所组成。结果初步说明,盘红细胞中HbA₂可能与HbA结合存在。两者可能有相互作用,也许这是产生血红蛋白A₂现象的原因。     

NO和H2O2诱导大豆根尖和边缘细胞耐铝反应的作用

 NO和H₂O₂是参与植物抗非生物胁迫反应的重要信号分子, 为了确定NO和H₂O₂在大豆(Glycine max)根尖和根边缘细胞(root border cells, RBCs)耐铝反应中的作用及其相互关系, 以‘浙春3号’大豆为材料, 研究了铝毒胁迫下大豆根尖内源NO和H₂O₂的变化, 以及外源NO和H₂O₂诱导大豆根尖和RBCs的耐铝反应。结果表明, 50 μmol·L^–1 Al处理48 h显著抑制大豆根的伸长, 提高Al在根尖的积累, 同时显著增加根尖内源NO和H₂O₂含量。施加0.25 mmol·L^–1外源NO供体亚硝基铁氰化钠(Na₂[Fe(CN)₅NO]·2H₂O, sodium nitroprusside, SNP)和0.1 mmol·L^–1H₂O₂, 能有效地缓解Al对大豆根伸长的抑制、根尖Al积累和RBCs 的死亡, 该缓解作用可以被0.05 mmol·L^–1 NO清除剂2-(4- 羧基苯)-4,4,5,5- 四甲基咪唑-1- 氧-3- 氧化物, 钾盐(C₁₄H₁₆N₂O₄·K, carboxy-PTIO, cPTIO)和150 U·mL^–1 H₂O₂清除酶(catalase, CAT)逆转。并且外源NO能够显著促进根尖H₂O₂的积累, 而外源H₂O₂对根尖NO的含量无显著影响。这表明NO和H₂O₂是诱导大豆根尖及RBCs耐铝反应的两种信号分子, NO可能通过调控H₂O₂的形成, 进而诱导大豆根尖及RBCs的耐铝反应。     

胞外ATP对AlCl3诱导的细胞死亡过程中胞内H2O2和Ca2+水平的影响及其生理机制分析

该实验以烟草悬浮细胞 BY 2 为材料,在烟草悬浮细胞中分别加入0.05、0.10、0.15、0.20 mmol·L^-1AlCl₃,以等体积去离子水处理的悬浮细胞液为对照,并依据前述实验结果选择0.15 mmol·L^-1 AlCl₃,分别添加5 mmol·L^-1 DMTU(H₂O₂ 抑制剂)、20 μmol·L^-1CaCl₂、15 μmol·L^-1 LaCl₃(Ca²⁺通道抑制剂)和50 μmol·L^-1 ATP设计多项处理,分析胞外ATP(eATP)对铝离子(Al³⁺)胁迫引起的植物细胞死亡及其胞内H₂O₂、Ca²⁺的影响,以揭示Al³⁺胁迫下植物调节细胞死亡的可能机制,进一步扩展对eATP功能的认知。结果显示：(1)随着 AlCl₃ 胁迫浓度的提高,细胞死亡水平和胞内H₂O₂水平上升,而胞内Ca²⁺和eATP水平则逐渐降低。(2)外援施加H₂O₂抑制剂 DMTU(二甲基硫脲)和Ca²⁺能够有效缓解AlCl₃诱导的细胞死亡水平的上升;而Ca²⁺通道抑制剂LaCl₃(三氯化镧)则加剧了AlCl₃胁迫下的细胞死亡。(3)在AlCl₃胁迫下对细胞添加外源ATP,能够缓解AlCl₃胁迫下胞内H₂O₂水平上升和Ca²⁺水平下降的同时,并显著降低AlCl₃胁迫导致的细胞死亡。研究表明, Al³⁺以剂量依赖的模式提升细胞死亡和细胞内H₂O₂的水平并降低胞内Ca²⁺和eATP水平,AlCl₃诱导的细胞死亡受到H₂O₂和Ca²⁺水平变化的调节,eATP可以通过调节H₂O₂与Ca²⁺水平缓解AlCl₃诱导的细胞死亡。推测Al³⁺胁迫可能通过抑制钙离子通道而破坏了细胞内H₂O₂和Ca²⁺之间的协同关系,外源ATP对Al³⁺诱导H₂O₂上升的缓解作用可能是由于其提升了细胞的抗氧化能力。     

SelS高表达保护人脐静脉内皮细胞免于H2O2诱导的细胞损伤

采用以下方法探讨SelS在内皮细胞中的表达和作用：将SelS基因克隆到真核表达载体pLNCX2，RT-PCR、XhoⅠ/ClaⅠ双酶切以及DNA序列分析验证目的基因；利用脂质体转染技术将pLNCX2-SelS或pLNCX2转染至人脐静脉内皮细胞(ECV₃₀₄细胞)，RT-PCR检测重组基因SelS的表达；MTT方法检测转染后过氧化氢(H₂O₂)对内皮细胞增殖能力的影响；硫代巴比妥酸法测定暴露于H₂O₂中不同转染组细胞脂质过氧化产物丙二醛含量. 结果表明：成功构建真核表达载体pLNCX2-SelS；转染后重组SelS mRNA表达水平是内源性水平的1.76倍；H₂O₂对ECV₃₀₄细胞损伤后，高表达SelS组细胞活性增强、H₂O₂诱导产生的丙二醛减少. 上述结果表明，高表达SelS可保护内皮细胞免于H₂O₂诱导的细胞损伤，其作用机制与抗氧化有关.     

Genetic Analysis of Growth Inhibition of Yeast Cells Caused by Expression of Aspergillus oryzae RNase T1

Even though most fungal hydrolytic enzymes have been successfully secreted in S. cerevisiae cells by expression of corresponding cDNA, overexpression of A. oryzae RNase T1 causes severe growth inhibition in yeast. We observed that yeast strains carrying RNase T1 cDNA under control of the GAL1 promoter with a single-copy vector were able to grow on galactose medium while those with a multi-copy vector were not. It was found that overexpression of three mutated versions of RNase T1 with low enzymatic activity did not affect the growth. We also observed that expression of RNase T1 without a signal sequence severely inhibited growth of the transformant even on the single-copy plasmid. Subcellular fractionation showed that overexpressed myc-tagged RNase T1 was localized in the membrane fraction. In the yeast secretory pathway, while the mutants defective in translocation into the ER, ER-Golgi trafficking and vacuole formation had severe growth inhibition during expression of RNase T1 from the single-copy plasmid. These results suggest that a mislocalization of active RNase T1 in cytosol by overflow from the secretory apparatus has toxic effects on the host cells.     

Natural Killer Cells Control Tumor Growth by Sensing a Growth Factor

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Control of Francisella tularensis Intracellular Growth by Pulmonary Epithelial Cells

The virulence of F. tularensis is often associated with its ability to grow in macrophages, although recent studies show that Francisella proliferates in multiple host cell types, including pulmonary epithelial cells. Thus far little is known about the requirements for killing of F. tularensis in the non-macrophage host cell types that support replication of this organism. Here we sought to address this question through the use of a murine lung epithelial cell line (TC-1 cells). Our data show that combinations of the cytokines IFN-γ, TNF, and IL-17A activated murine pulmonary epithelial cells to inhibit the intracellular growth of the F. tularensis Live Vaccine Strain (LVS) and the highly virulent F. tularensis Schu S4 strain. Although paired combinations of IFN-γ, TNF, and IL-17A all significantly controlled LVS growth, simultaneous treatment with all three cytokines had the greatest effect on LVS growth inhibition. In contrast, Schu S4 was more resistant to cytokine-induced growth effects, exhibiting significant growth inhibition only in response to all three cytokines. Since one of the main antimicrobial mechanisms of activated macrophages is the release of reactive nitrogen intermediates (RNI) via the activity of iNOS, we investigated the role of RNI and iNOS in Francisella growth control by pulmonary epithelial cells. NOS2 gene expression was significantly up-regulated in infected, cytokine-treated pulmonary epithelial cells in a manner that correlated with LVS and Schu S4 growth control. Treatment of LVS-infected cells with an iNOS inhibitor significantly reversed LVS killing in cytokine-treated cultures. Further, we found that mouse pulmonary epithelial cells produced iNOS during in vivo respiratory LVS infection. Overall, these data demonstrate that lung epithelial cells produce iNOS both in vitro and in vivo, and can inhibit Francisella intracellular growth via reactive nitrogen intermediates.     

鸟氨酸脱羧酶抗酶抑制因子-1高表达抑制黑素瘤细胞在小鼠体内的生长

鸟氨酸脱羧酶抗酶抑制因子-1(ornithine decarboxylase antienzyme inhibitor-1,OAZI-1)是细胞内调节多胺代谢的重要蛋白质因子。已有研究发现,OAZI-1高表达的黑素瘤细胞在体外能更有效地被抗原提呈细胞识别和吞噬,提示OAZI-1在肿瘤免疫治疗中具有潜在的应用价值。为进一步分析OAZI-1高表达对黑素瘤细胞在小鼠体内生长的影响,高表达OAZI-1的黑素瘤细胞(B16/OAZI-1)被接种到实验小鼠体内,结果发现,接种瘤出现先成瘤随后逐渐消退的现象,至第24 d时,接种瘤的平均体积为36±25 mm3~,而对照细胞接种瘤的平均体积为326±309 mm~3。为探索上述现象的机制,随后分析了B16/OAZI-1在小鼠体内诱导的抗肿瘤免疫效应,结果发现:1)B16/OAZI-1接种显著增加了小鼠脾脏细胞对B16-F1瘤细胞的杀伤活性;2)源于B16-F1的细胞抗原能更有效地促进B16/OAZI-1接种小鼠脾脏细胞的增殖;3)B16/OAZI-1接种小鼠的脾脏细胞具有更强的分泌IFN-γ的能力;4)当在预接种B16/OAZI-1 30 d后的小鼠体内再次接种B16-F1活细胞时,新接种瘤细胞的生长受到显著抑制,小鼠的存活率增加。上述研究结果提示,高表达OAZI-1的黑素瘤细胞在实验动物体内的生长受到显著抑制,其机制可能与OAZI-1能促进肿瘤抗原提呈和诱导抗肿瘤免疫效应相关。     

重组人碱性成纤维细胞生长因子(bFGF)融合蛋白的高效表达及鉴定

碱性成纤维细胞生长因子（ｂＦＧＦ）参与了许多细胞生长和分化的调控过程。本文采用重组ＤＮＡ技术在大肠杆菌中高效表达了人ｂＦＧＦ。首先将编码人ｂＦＧＦ基因克隆到ｐＸＴ表达载体中与其上游的一短Ｓ导肽共一阅读框架,ｂＦＧＦ基因的表达受强的Ｔ７启动子调控。采用ＢＬ２１（ＤＥ３）大肠杆菌作为宿主菌,用ＩＰＴＧ诱导ＢＬ２１（ＤＥ３）细菌合成的Ｔ７ＲＮＡ聚合酶,后者可催化高水平的ｂＦＧＦ基因表达,其ｂＦＧＦ产量可占总菌体蛋白的４２.５％。采用肝素Ｓｅｐｈａｒｏｓｅ一步亲和层析法直接从诱导后的细菌裂解产物中得到纯化的重组人ｂＦＧＦ蛋白。经Ｗｅｓｔｅｒｎ印迹分析证明该蛋白可被人ｂＦＧＦ特异性单克隆抗体所识别。进一步研究证明该蛋白具有刺激ＮＲ６Ｒ－３Ｔ３成纤维细胞增殖的生物学活性,并且这一活性可被人ｂＦＧＦ特异性中和抗体所中和。     

Notch途径与宫颈癌细胞系的增殖调控

近年来在许多肿瘤细胞系中发现Notch基因的表达失常,失控的Notch信号对维持肿瘤细胞表型性起着重要作用。在宫颈癌细胞中,异常上调的Notch信号通路由人乳头瘤病毒(HPV)相关蛋白“E6/7”介导,并能与之发生协同作用维持肿瘤的生长及异型性,另一方面,激活的Notch1又能通过抑制Fos蛋白家族进而抑制“E6/7”的表达,并能通过抑制E47蛋白引起细胞增殖抑制。结合对不同时期宫颈癌细胞的研究结果,目前认为低水平的Notch1表达对维持发生癌变的角质细胞的生存相当重要,过多或过少的Notch1信号都会对细胞增殖造成负面影响。     

Nerve Growth Factor Promotes Neurite Regeneration in PC12 Cells by Translational Control

Abstract: When PC12 cells are primed with nerve growth factor (NGF) for periods of ≥1 week, they acquire the ability to regenerate neurites rapidly in response to NGF. It is not known how NGF promotes this regeneration, but it does not require ongoing RNA synthesis. Previous studies have suggested that NGF directs the accumulation of precursor molecules that are rapidly assembled to form the regenerated neurites. To address the nature of these precursor molecules, we have treated PC12 cells with macromolecular synthesis inhibitors during the priming and regeneration phases of neurite growth. Here we show that NGF promotes neurite regeneration by inducing the synthesis of new proteins. These proteins are encoded by short-lived mRNAs that are generated during the NGF priming period. The isolation and identification of these mRNAs will allow a further understanding of how NGF promotes neurite regeneration.     

Growth Control in Colon Epithelial Cells: Gadolinium Enhances Calcium-Mediated Growth Regulation

Gadolinium, a member of the lanthanoid family of transition metals, interacts with calcium-binding sites on proteins and other biological molecules. The overall goal of the present investigation was to determine if gadolinium could enhance calcium-induced epithelial cell growth inhibition in the colon. Gadolinium at concentrations as low as 1?C5???M combined with calcium inhibits proliferation of human colonic epithelial cells more effectively than calcium alone. Gadolinium had no detectable effect on calcium-induced differentiation in the same cells based on change in cell morphology, induction of E-cadherin synthesis, and translocation of E-cadherin from the cytosol to the cell surface. When the colon epithelial cells were treated with gadolinium and then exposed to increased calcium concentrations, movement of extracellular calcium into the cell was suppressed. In contrast, gadolinium treatment had no effect on ionomycin-induced release of stored intracellular calcium into the cytoplasm. Whether these in vitro observations can be translated into an approach for reducing abnormal proliferation in the colonic mucosa (including polyp formation) is not known. These results do, however, provide an explanation for our recent findings that a multi-mineral supplement containing all of the naturally occurring lanthanoid metals including gadolinium are more effective than calcium alone in preventing colon polyp formation in mice on a high-fat diet.     

拟南芥AtLH基因过量表达引起叶向下性卷曲和晚开花

AtLH基因是BcpLH基因在拟南芥(Arapsis thaliana L.)中的同源基因,含有两个编码双链RNA结合蛋白的结构域.在大白菜叶球发育过程中,BcpLH基因与包叶的卷曲有关.为研究AtLH的基因对叶卷曲这一重要生物学现象的调控作用,构建了35S:AtLH基因的正义表达载体并转化拟南芥.与野生型比较页言,转基因植株的花和叶中AtLH的表达量有显著增加,成为AtLH基因过量的植株.这些植株的莲座叶向外或向下卷曲,呈现明显的偏上性生长;而且抽苔和开花时间延迟;在营养生长期其短缩茎的叶腑处着生数个侧茎,表现为顶端优势减弱;在生殖生长期二级花序减少使得主花序更加发达,表现为顶端优势增强,转基因植株对激素的敏感性改变,IAA剌激根生长的作用增强,ABA抑制根生长的作用减弱.由此可见,AtLH基因的过量表达可引起转基因植株的叶片向下卷曲.     

拟南芥AtLH基因过量表达引起叶向下性卷曲和晚开花(英文)

AtLH基因是BcpLH基因在拟南芥(Arabidopsis thealiana L.)中的同源基因,含有两个编码双链RNA结合蛋白的结构域。在大白菜叶球发育过程中,BcpLH基因与包叶的卷曲有关。为研究AtLH基因对叶卷曲这一重要生物学现象的调控作用,构建了35S:AtLH基因的正义表达载体并转化拟南芥。与野生型比较而言,转基因植株的花和叶中AtLH的表达量有显著增加,成为AtLH基因过量表达的植株。这些植株的莲座叶向外或向下卷曲,呈现明显的偏上性生长;而且抽苔和开花时间延迟;在营养生长期其短缩茎的叶腋处着生数个侧茎,表现为顶端优势减弱;在生殖生长期二级花序减少使得主花序更加发达,表现为顶端优势增强;转基因植株对激素的敏感性改变,IAA刺激根生长的作用增强,ABA抑制根生长的作用减弱。由此可见,AtLH基因的过量表达可引起转基因植株的叶片向下卷曲。