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.     

超微粒TiO2对U937细胞光杀伤效应及机理研究

超微粒TiO₂经光催化氧化后对U937白血病细胞有明显的杀伤作用,DNA琼脂糖凝胶电泳图证明了光激发TiO₂能够损伤细胞内的DNA,从而导致细胞死亡,提出了一种杀伤癌细胞的新思路.     

PKCγ过表达诱导C3H10T1/2细胞生长失控的初探

通过DNA重组构建蛋白激酶C_γ(PKC_γ)亚类的重组质粒并经基因转染技术和DNA印迹、蛋白质印迹与PKC活性分析,获得了过表达PKC_γ的C₃H₁₀T_1/2细胞——NCP4.NCP4细胞生长速率提高,流式细胞光度术检测表明,NCP4细胞G1期百分率下降,S期和G2+M期百分率升高,与对照组细胞相比,血清依赖性明显下降,贴壁依赖性降低,在软琼脂中形成小集落,出现部分转化表型.进一步检测,首次观察到NCP4细胞中癌基因c-sis表达明显增强,这可能是NCP4细胞血清依赖性下降的分子机理之一.实验表明,在正常C₃H₁₀T_1/2细胞中PKC_γ的过表达可直接导致细胞增殖加速并可诱导出现部分转化特征.     

细胞氧化损伤时8-羟基鸟嘌呤的测定

利用H₂O₂易通过细胞膜而到达核这一特点,初步探讨了不同浓度H₂O₂对HL-60细胞DNA的氧化损伤程度.发现H₂O₂浓度在0.4 mmol/L以上时,作用8～24 h可以用气相色谱/火焰离子检测器(GC/FID)检测到氧化损伤标志产物——8-羟基鸟嘌呤(8-oh-G),并观测到在0.4～0.8 mmol/L H₂O₂作用一定时间时,8-羟基鸟嘌呤含量随H₂O₂浓度升高而升高.     

Mg2＋对阿霉素引起心肌线粒体F1F0变化的保护

抗肿瘤药物阿霉素(ADM)对心肌线粒体F₁F₀-复合体呈现抑制而对F₁-ATPase无抑制,这表明ADM可能是通过膜脂起作用的,适当浓度Mg²⁺能降低ADM对复合体的抑制.经 ³¹P-NMR和标记荧光探针NBD-PE,DPH,MC-540以及内源荧光等的测定,结果表明ADM可能首先通过诱导F₁F₀膜脂形成非双层脂结构,继而影响了膜脂的堆积程度和流动性,进而引起F₁F₀-复合体酶蛋白构象的改变,最终导致酶活力的降低.Mg^2＋则可能由于与ADM竞争与心磷脂的结合,而对ADM引起F₁F₀的变化产生保护作用.     

NaHCO3胁迫对紫根水葫芦形态学指标和光合参数的影响

为研究NaHCO₃胁迫对紫根水葫芦的形态学指标及光合参数的影响,该文以紫根水葫芦为材料,采用不同浓度碱性盐NaHCO₃溶液处理成株紫根水葫芦,测定在NaHCO₃胁迫下紫根水葫芦的植株株高、根长、根冠比、生物量、含水量和光合参数[净光合速率(P_n)、胞间CO₂浓度(C_i)、蒸腾速率(T_r)、气孔导度(G_s)]。结果表明:紫根水葫芦在20 mmol·L^-1 NaHCO₃浓度下的水溶液pH值最为平缓; 在低浓度NaHCO₃溶液中(≤40 mmol·L^-1),相比CK,紫根水葫芦的形态学指标呈现增长或无显著影响情况,而在高浓度NaHCO₃溶液中(≥60 mmol·L^-1),随着NaHCO₃浓度的升高,紫根水葫芦形态学指标显著降低,且与NaHCO₃浓度呈负相关; NaHCO₃胁迫对紫根水葫芦的光合参数影响显著,随着NaHCO₃浓度的增加及试验处理时间的延长,紫根水葫芦的P_n呈持续下降的趋势,C_i、T_r和G_s整体呈上升趋势,其光合作用受到的主要是非气孔限制。综合分析显示,紫根水葫芦具有一定的耐NaHCO₃能力,能正常生存在不超过40 mmol·L^-1 NaHCO₃浓度的水体中,且能改善低NaHCO₃浓度下的水体pH值。     

应用稳定同位素技术分析华北部分地区第三代棉铃虫虫源性质

玉米等C₄植物被认为是华北Bt棉种植区内第三代棉铃虫最重要的天然庇护所,但尚缺乏直接证据。连续2a(2006-2007年)利用杨树把诱集棉铃虫成虫,进行碳稳定同位素比值的测定,并结合棉铃虫成虫捕获时间、虫源的数量比例等,评估C₄植物在华北第三代棉铃虫期间的庇护所功能。结果表明,第三代棉铃虫成虫来源于C₄植物(玉米)的为40.5%-56.8%,与C₃来源的数量上大体相当。但C₄来源的成虫羽化时间比C₃来源的个体明显滞后,呈现出先少后多的特点。结果提示,C₄植物确实是华北第三代棉铃虫重要的庇护所,但存在着时间上与C₃来源的成虫交配不同步而失效的风险;结果建议玉米等天然庇护所作物的种植不仅在面积上要足够,而且播种时间上要充分考虑C₄植物(玉米)来源的敏感棉铃虫个体的发育与C₃植物寄主来源个体的同步性。     

高大气CO2浓度下小麦旗叶光合能量利用对氮素和光强的响应

采用开顶式气室盆栽培养小麦,设计2个大气CO₂浓度、2个光照强度和2个氮水平的组合处理,通过测定小麦叶片光合速率-胞间CO₂浓度响应曲线和叶绿素荧光参数,来测算小麦叶片光化学速率、光合电子传递速率以及叶绿体磷酸丙糖利用效率(TPU)等参数,研究施氮量和光强对高大气CO₂浓度下小麦旗叶光合能量传递与分配的影响,以阐明全球气候变化下植物光合能量分配对光合作用适应性下调的作用机制及其氮素调控。结果表明,大气CO₂浓度升高后小麦叶片的光呼吸电子传递速率(J₀)和Rubisco氧化速率(V₀)显著下降;光合电子流的光化学传递速率(J_C)、Rubisco羧化速率(V_C)和TPU则明显升高,而且施氮后变化幅度加大;小麦叶片J_C/J_F(PSⅡ反应中心总电子流速率)和TPU/V_C显著增加,经过PSⅡ反应中心的电子流更多地进入碳同化过程,表现较高的光合速率(P_n)。遮荫提高了叶片光化学速率和PSⅡ反应中心总电子流速率(J_F),这一作用在低氮叶片尤为突出,但使得J₀和V₀明显升高,并显著降低J_C/J_F,所以P_n明显下降。正常光照条件下,增施氮素可提高小麦叶片的J_F、J_C、V_C和TPU,并使高大气CO₂浓度下J₀和V₀较正常大气CO₂浓度处理显著降低,有效地提高了植物叶片对光能的利用效率;遮荫后高大气CO₂浓度下小麦叶片J_C、V_C、TPU、J_C/J_F和TPU/V_C显著高于正常大气CO₂浓度处理,而且这一变化不受氮素水平的显著调节。因此,氮素在高大气CO₂浓度下对小麦叶片光合能量利用的调节因光强而异,正常光照下可显著改善小麦叶片对光合能量的利用状况,而遮荫后这一作用减弱。     

竹红菌乙素作猝灭剂研究Fo构象方法的建立

线粒体F₁F_o复合体F_o部分a亚基的色氨酸荧光可被竹红菌乙素(hypocrellin B, HB)猝灭.不同温度下测定Stern-Volmer图的结果显示,猝灭常数(K_sv)随温度的增加而加大,时间衰变荧光的结果显示,荧光寿命随HB浓度的增加而减小,加入不同浓度的HB, F₁F_o复合体的吸收峰没有位移.这些实验结果支持动态猝灭机理.HB还具有有效猝灭浓度低,不影响酶的活力;在脂相和水相的分布比率可高达16 560∶1;实验操作简便等优点.因此HB可作为理想的疏水相荧光猝灭剂,研究与膜结合的F₁F_o复合体中镶嵌于膜脂内F_o的构象变化.     

三氧化二砷下调MG-63骨肉瘤细胞IEX-1基因表达的转录调控机制研究

三氧化二砷(arsenic trioxide, As₂O₃)是中国传统中药砒霜的主要有效成分,最早应用于血液系统肿瘤的治疗,随后研究表明其对实体瘤也具有抑制细胞增殖并诱导凋亡的作用．早期研究发现,1.0 μmol/L的As₂O₃可以体外诱导骨肉瘤细胞系MG-63细胞凋亡,进一步的cDNA芯片分析、RT-PCR、RNA印迹证实细胞凋亡与As2O3干预后IEX-1基因表达下调有关．IEX-1为早期诱导应答基因,调节细胞生长和凋亡．通过荧光素酶分析,EMSA、蛋白质印迹等实验,发现As₂O₃干预骨肉瘤细胞系MG-63后能诱导p53蛋白表达上调,增加的p53蛋白通过与IEX-1的启动子结合,转录抑制IEX-1的转录,导致IEX-1基因表达下调．进一步证实了IEX-1与骨肉瘤的重要关系,同时也阐明As₂O₃诱导IEX-1基因表达下调的转录调控机制．     

A predicted geranylgeranyl reductase reduces the ω-position isoprene of dolichol phosphate in the halophilic archaeon, Haloferax volcanii

In N-glycosylation in both Eukarya and Archaea, N-linked oligosaccharides are assembled on dolichol phosphate prior to transfer of the glycan to the protein target. However, whereas only the α-position isoprene subunit is saturated in eukaryal dolichol phosphate, both the α- and ω-position isoprene subunits are reduced in the archaeal lipid. The agents responsible for dolichol phosphate saturation remain largely unknown. The present study sought to identify dolichol phosphate reductases in the halophilic archaeon, Haloferax volcanii. Homology-based searches recognize HVO_1799 as a geranylgeranyl reductase. Mass spectrometry revealed that cells deleted of HVO_1799 fail to fully reduce the isoprene chains of H. volcanii membrane phospholipids and glycolipids. Likewise, the absence of HVO_1799 led to a loss of saturation of the ω-position isoprene subunit of C₅₅ and C₆₀ dolichol phosphate, with the effect of HVO_1799 deletion being more pronounced with C₆₀ dolichol phosphate than with C₅₅ dolichol phosphate. Glycosylation of dolichol phosphate in the deletion strain occurred preferentially on that version of the lipid saturated at both the α- and ω-position isoprene subunits.     

Cholesterol-mediated membrane surface area dynamics in neuroendocrine cells

How cholesterol, a key membrane constituent, affects membrane surface area dynamics in secretory cells is unclear. Using methyl-β-cyclodextrin (MβCD) to deplete cholesterol, we imaged melanotrophs from male Wistar rats in real-time and monitored membrane capacitance (C_m), fluctuations of which reflect exocytosis and endocytosis. Treatment with MβCD reduced cellular cholesterol and caused a dose-dependent attenuation of the Ca²⁺-evoked increase in C_m (IC₅₀ = 5.3 mM) vs. untreated cells. Cytosol dialysis of MβCD enhanced the attenuation of C_m increase (IC₅₀ = 3.3 mM), suggesting cholesterol depletion at intracellular membrane sites was involved in attenuating exocytosis. Acute extracellular application of MβCD resulted in an immediate C_m decline, which correlated well with the cellular surface area decrease, indicating the involvement of cholesterol in the regulation of membrane surface area dynamics. This decline in C_m was three-fold slower than MβCD-mediated fluorescent cholesterol decay, implying that exocytosis is the likely physiological means for plasma membrane cholesterol replenishment. MβCD had no effect on the specific C_m and the blockade of endocytosis by Dyngo 4a, confirmed by inhibition of dextran uptake, also had no effect on the time-course of MβCD-induced C_m decline. Thus acute exposure to MβCD evokes a C_m decline linked to the removal of membrane cholesterol, which cannot be compensated for by exocytosis. We propose that the primary contribution of cholesterol to surface area dynamics is via its role in regulated exocytosis.     

The Inhibitor Protein (IF1) of the F1F0-ATPase Modulates Human Osteosarcoma Cell Bioenergetics

The bioenergetics of IF₁ transiently silenced cancer cells has been extensively investigated, but the role of IF₁ (the natural inhibitor protein of F₁F₀-ATPase) in cancer cell metabolism is still uncertain. To shed light on this issue, we established a method to prepare stably IF₁-silenced human osteosarcoma clones and explored the bioenergetics of IF₁ null cancer cells. We showed that IF₁-silenced cells proliferate normally, consume glucose, and release lactate as controls do, and contain a normal steady-state ATP level. However, IF₁-silenced cells displayed an enhanced steady-state mitochondrial membrane potential and consistently showed a reduced ADP-stimulated respiration rate. In the parental cells (i.e. control cells containing IF₁) the inhibitor protein was found to be associated with the dimeric form of the ATP synthase complex, therefore we propose that the interaction of IF₁ with the complex either directly, by increasing the catalytic activity of the enzyme, or indirectly, by improving the structure of mitochondrial cristae, can increase the oxidative phosphorylation rate in osteosarcoma cells grown under normoxic conditions.     

H2O2 induces rapid biophysical and permeability changes in the plasma membrane of Saccharomyces cerevisiae

In Saccharomyces cerevisiae, the diffusion rate of hydrogen peroxide (H₂O₂) through the plasma membrane decreases during adaptation to H₂O₂ by means of a mechanism that is still unknown. Here, evidence is presented that during adaptation to H₂O₂ the anisotropy of the plasma membrane increases. Adaptation to H₂O₂ was studied at several times (15min up to 90min) by applying the steady-state H₂O₂ delivery model. For wild-type cells, the steady-state fluorescence anisotropy increased after 30min, or 60min, when using 2-(9-anthroyloxy) stearic acid (2-AS), or diphenylhexatriene (DPH) membrane probe, respectively. Moreover, a 40% decrease in plasma membrane permeability to H₂O₂ was observed at 15min with a concomitant two-fold increase in catalase activity. Disruption of the ergosterol pathway, by knocking out either ERG3 or ERG6, prevents the changes in anisotropy during H₂O₂ adaptation. H₂O₂ diffusion through the plasma membrane in S. cerevisiae cells is not mediated by aquaporins since the H₂O₂ permeability constant is not altered in the presence of the aquaporin inhibitor mercuric chloride. Altogether, these results indicate that the regulation of the plasma membrane permeability towards H₂O₂ is mediated by modulation of the biophysical properties of the plasma membrane.     

The crystal structure of the C₂A domain of otoferlin reveals an unconventional top loop region

Otoferlin (Otof), whose genetic mutations cause profound deafness in humans, is a protein composed of at least six C₂ domains, which are known as Ca²⁺-binding and phospholipid-binding regions. Mammalian ferlin proteins are proposed to act in membrane fusion events, with Otof being specifically required for exocytosis in auditory hair cells. Ferlin C₂ domains exhibit a rather low level of sequence similarity to those of synaptotagmins, protein kinase C isoforms, or phospholipases. Here, we report the crystal structure of the N-terminal C₂ domain of Otof (C₂A) at 1.95-Å resolution. In contrast to previous predictions, we found that this C₂ domain is complete with eight β-strands. Comparing the structure of Otof C₂A to those of other C₂ domains revealed one top loop in Otof to be significantly shorter. This results in a depression of the surface, which is positively charged for the Otof C₂A domain, and contrasts with the head-like protrusion surrounded by a negatively charged “neck” typically found in other C₂ domains. Isothermal titration calorimetry and circular dichroism spectroscopy studies confirmed that Otof C₂A is unable to bind Ca²⁺, while the synaptotagmin-1 C₂A domain exhibited Ca²⁺ binding under the same conditions. Furthermore, floatation assays revealed a failure of Otof C₂A to bind to phospholipid membranes. Accordingly, no positively charged β-groove-like surface structure, which is known to bind phosphatidylinositol-4,5-bisphosphate in other C₂ domains, was found at the respective position in Otof C₂A. Taken together, these data demonstrate that the Otof C₂A domain differs structurally and functionally from other C₂ domains.     

A comparative immunocytochemical localization study of phosphoenolpyruvate carboxylase in leaves of higher plants

The intracellular localization of phosphoenolpyruvate (PEP) carboxylase in plants belonging to the C₄, Crassulacean acid metabolism (CAM) and C₃ types was invetigated using an immunocytochemical method with an immune serum raised against the sorghum leaf enzyme. The plants studied were sorghum, maize (C₄ type), kalanchoe (CAM type), french bean, and spinach (C₃ type). In the green leaves of C₄ plants, it was shown that the carboxylase was located in the mesophyll and stomatic cells, being largely cytosolic in the mesophyll cells. Similarly, in CAM plants, the enzyme was found mainly outside the chloroplasts. In contrast, in C₃ plants, the PEP carboxylase appeared to be distributed between the cytosol and the chloroplasts of foliar parenchyma. Examination of sections from etiolated leaves showed fluorescence emission from etioplasts and cytosol for the parenchyma of french bean as well as for the bundle sheath and mesophyll of sorghum leaves. This data indicated that during the greening process photoregulation and evolution of PEP carboxylase is dependent on the tissue and on the metabolic type of the plant considered.Abbreviations CAM Crassulacean acid metabolism - PEP phosphoenolpyruvate     

A possible role of lysophospholipids produced by calcium-independent phospholipase A2 in membrane-raft budding and fission

Phospholipase A₂ (PLA₂) not only plays a role in the membrane vesiculation system but also mediates membrane-raft budding and fission in artificial giant liposomes. This study aimed to demonstrate the same effects in living cells. Differentiated Caco-2 cells were cultured on filter membranes. MDCK cells were challenged with Influenza virus. The MDCK cultures were harvested for virus titration with a plaque assay. Alkaline phosphatase (ALP), a membrane-raft associated glycosylphosphatidylinositol (GPI)-anchored protein, was 70% released by adding 0.2 mmol/l lysophosphatidylcholine, which was abolished by treatment with a membrane-raft disrupter, methyl-β-cyclodextrin. Activation of calcium-independent PLA₂ (iPLA₂) by brefeldin A increased the apical release of ALP by approximately 1.5-fold (p < 0.01), which was blocked by PLA₂ inhibitor bromoenol lactone (BEL). BEL also reduced Influenza virus production into the media (< 10%) in the MDCK culture. These results suggest that cells utilize inverted corn-shaped lysophospholipids generated by PLA₂ to modulate plasma membrane structure and assist the budding of raft-associated plasma membrane particles, which virus utilizes for its budding. Brush borders are enriched with membrane-rafts and undergo rapid turnover; thus, PLA₂ may be involved in the regulatory mechanism in membrane dynamism. Further, iPLA₂ may provide a therapeutic target for viral infections.     

Clustering of sialylated glycosylphosphatidylinositol anchors mediates PrP-induced activation of cytoplasmic phospholipase A2 and synapse damage

Precisely how the accumulation of PrP^Sc causes the neuronal degeneration that leads to the clinical symptoms of prion diseases is poorly understood. Our recent paper showed that the clustering of specific glycosylphosphatidylinositol (GPI) anchors attached to PrP proteins triggered synapse damage in cultured neurons. First, we demonstrated that small, soluble PrP^Sc oligomers caused synapse damage via a GPI-dependent process. Our hypothesis, that the clustering of specific GPIs caused synapse damage, was supported by observations that cross-linkage of PrP^C, either chemically or by monoclonal antibodies, also triggered synapse damage. Synapse damage was preceded by an increase in the cholesterol content of synapses and activation of cytoplasmic phospholipase A₂ (cPLA₂). The presence of a terminal sialic acid moiety, a rare modification of mammalian GPI anchors, was essential in the activation of cPLA₂ and synapse damage induced by cross-linked PrP^C. We conclude that the sialic acid modifies local membrane microenvironments (rafts) surrounding clustered PrP molecules resulting in aberrant activation of cPLA₂ and synapse damage. A recent observation, that toxic amyloid-β assemblies cross-link PrP^C, suggests that synapse damage in prion and Alzheimer diseases is mediated via a common molecular mechanism, and raises the possibility that the pharmacological modification of GPI anchors might constitute a novel therapeutic approach to these diseases.     

The high turnover Drosophila multidrug resistance-associated protein shares the biochemical features of its human orthologues

DMRP, an ABC transporter encoded by the dMRP/CG6214 gene, is the Drosophila melanogaster orthologue of the “long” human multidrug resistance-associated proteins (MRP1/ABCC1, MRP2/ABCC2, MRP3/ABCC3, MRP6/ABCC6, and MRP7/ABCC10). In order to provide a detailed biochemical characterisation we expressed DMRP in Sf9 insect cell membranes. We demonstrated DMRP as a functional orthologue of its human counterparts capable of transporting several human MRP substrates like β-estradiol 17-β-d-glucuronide, leukotriene C₄, calcein, fluo3 and carboxydichlorofluorescein. Unexpectedly, we found DMRP to exhibit an extremely high turnover rate for the substrate transport as compared to its human orthologues. Furthermore, DMRP showed remarkably high basal ATPase activity (68-75 nmol P_i/mg membrane protein/min), which could be further stimulated by probenecid and the glutathione conjugate of N-ethylmaleimide. Surprisingly, this high level basal ATPase activity was inhibited by the transported substrates. We discussed this phenomenon in the light of a potential endogenous substrate (or activator) present in the Sf9 membrane.     

不同BR施用方式诱导黄瓜幼苗对Ca(NO_3)_2胁迫抗性的研究

为探讨外源油菜素内酯(brassinosteroid,BR)诱导黄瓜幼苗对Ca(NO3)2胁迫抗性的效果,研究了3种外源BR施用方法(0.01mg·L-1 BR浸种、0.1mg·L-1 BR喷叶及其二者结合施用)对Ca(NO3)2胁迫(60mmol·L-1)下黄瓜幼苗生长、生理活动以及光合作用的影响。结果表明:(1)3种外源BR方法处理后,Ca(NO3)2胁迫下的黄瓜幼苗株高、茎粗、展开叶片数、叶面积、干重含水量均显著提高,同时其叶片游离脯氨酸和可溶性糖含量上升,过氧化物酶活性提高,而其丙二醛(MDA)含量趋于无Ca(NO3)2胁迫对照的水平;(2)外源BR处理还提高了Ca(NO3)2胁迫下黄瓜幼苗的净光合速率、蒸腾速率和气孔导度,却抑制了Ca(NO3)2胁迫下胞间CO2浓度的升高。研究认为,适宜浓度的外源BR浸种和喷叶处理均可有效增强黄瓜幼苗渗透调节能力,降低细胞膜质过氧化伤害程度,提高抗氧化酶活性和光合效率,从而表现出对Ca(NO3)2胁迫的抗性,并以操作简便、用量极低的0.01mg·L-1 BR浸种方法效果最佳。