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.     

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.     

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.     

胞浆型磷脂酶A2介导弱氧化修饰低密度脂蛋白诱导的人脐静脉内皮细胞凋亡

探讨弱氧化修饰低密度脂蛋白(MM-LDL)能否诱导人脐静脉内皮细胞(HUVECs)凋亡以及胞浆型磷脂酶A₂(cPLA₂)在此过程中的作用.MTT法测定细胞存活率;相差显微镜、荧光显微镜和流式细胞仪检测细胞凋亡;³H-花生四烯酸(³H-AA)预标法测定PLA₂活性;蛋白质印迹检测cPLA₂磷酸化;激光共聚焦显微镜检测单个细胞内钙离子浓度的变化.结果表明,MM-LDL(100～300 mg/L)作用后的HUVECs呈现凋亡典型的形态特征,凋亡率随MM-LDL浓度的增加而上升.MM-LDL能引起胞内钙离子浓度增加,cPLA₂的活化及磷酸化.15 μmol/L AACOCF₃和5 mmol/L EGTA在抑制cPLA₂活性的同时,部分抑制MM-LDL诱导的HUVECs凋亡.加入外源性AA(50 μmol/L)能逆转AACOCF₃引起的凋亡抑制.结果提示,cPLA₂参与了MM-LDL诱导HUVECs凋亡的信号传递.     

神经节苷脂GM3对J6－2细胞蛋白质磷酸化的影响

通过研究神经节苷脂GM₃对国人单核样白血病细胞系J6-2细胞蛋白质磷酸化的影响,在[γ- ³²P]ATP,GM₃,ATP,Mg²⁺与J6-2细胞液及颗粒两部分共同反应,10min(30℃)体系中,观察到GM₃对两部分蛋白质磷酸化的调节作用.GM₃(100μmol/L)促进颗粒部分分子量为180 000,87 000,78 000,67 000,43 000及31 000的蛋白质磷酸化,促进胞液部分分子量为87 000及56 000的蛋白质磷酸化,而且能抑制70 000及43 000蛋白质磷酸化.由于GM₃已被前人证实能对J6-2细胞起分化作用,其作用时间长达4-6d,很可能GM₃对蛋白质磷酸化作用的调节是GM₃促分化作用的早期信号.     

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.     

无机磷影响叠氮钠对ATP合成酶合成活性的抑制

利用ADP和放射性磷直接合成ATP的方法,研究了无机磷(P_i)和叠氮钠对猪心线粒体ATP合成酶（F₁F_O-ATPase）ATP合成活性的影响.结果发现无机磷除作为合成ATP的底物参与F₁F_O-ATPase的合成反应外,还对F₁F_O-ATPase的合成活性呈现抑制作用,在1 mmol/L ADP存在时,随着P_i浓度由0.01～10 mmol/L增加,抑制合成作用越来越强.与叠氮钠在低浓度时(小于1 mmol/L)只抑制ATP水解,不影响ATP合成的观点不同.实验结果显示0.1 mmol/L叠氮钠表观激活F₁F_O-ATPase的ATP合成活性,且激活程度与反应体系中所加P_i的浓度呈负相关.当固定P_i浓度（0.1 mmol/L）后,随着叠氮钠浓度的增加表观激活程度也在变化,叠氮钠与磷浓度相等时表观激活程度最大,直至叠氮钠浓度接近0.5 mmol/L时,开始呈现表观抑制现象,叠氮钠浓度高于1 mmol/L之后,就出现解偶联现象.     

膜上斑点洁显示人红细胞b5还原酶活性

人红细胞NADH-细胞色素b₅还原酶是使高铁血红蛋白还原的主要酶类, 其缺陷将导致遗传性高铁血红蛋白血症. 目前, 主要通过分光光度法测定b₅还原酶活性. 我们将b₅还原酶抗体点于硝酸纤维膜上, 以此捕获并富集红细胞胞浆b₅还原酶. 有b₅还原酶活性的斑点用噻唑蓝染色. 此法简单直观, 可用于b₅还原酶的定性和半定量测定, 为遗传性高铁血红蛋白血症的诊断提供了一种新的实验手段.     

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．     

过氧化氢对培养心肌细胞损伤作用的研究

氧化应激时产生大量的自由基,造成心肌细胞的损伤.过氧化氢(H₂O₂)是有机体氧化代谢产物,同时是一种活性氧.应用不同浓度的H₂O₂,分别于不同作用时间,动态观察其对心肌细胞的损伤作用.从实验结果看到,低浓度的H₂O₂（＜0.1 mmol/L）作用2 h,使心肌细胞产生早期的生物化学的改变,如MDA产生堆积和细胞周期时相改变（G1期细胞增加,G2期细胞减少）,此时心肌酶基本无泄漏,心肌细胞的死亡率很低,HE形态学观察基本无改变;随着H₂O₂浓度的增加（1～5 mmol/L）和作用时间的延长,进一步诱导细胞损伤加剧,LDH释放和MDA积累明显升高,细胞死亡率也明显增加,已具有统计学意义.同时可观察到其病理形态学的坏死性改变;当10 mmol/L H₂O₂作用时,细胞大量死亡,形态学可见细胞极度收缩、脱落,形成大面积的细胞脱失区.因此,H₂O₂作为一种活性氧自由基,依其浓度和作用时间不同可造成不同程度的心肌细胞的损伤.辣根过氧化物酶作为一种自由基清除剂,可明显减少H₂O₂活性氧自由基对心肌细胞的损伤作用.     

Studies of the pyrolysis of tetraethylammonium tetrahydroborate

Tetraethylammonium tetrahydroborate, Et₄NBH₄, in suspension in refluxing decane-dodecane mixtures has been pyrolysed at temperatures between 175 and 190 °C. Et₃NBH₃, which is produced by partial decomposition of Et₄NBH₄, reacts with Et₄NBH₄ to give the intermediate Et₄NB₃H₈. Et₄NBH₄ and Et₃NBH₃ are also involved in the conversion of Et₄NB₃H_8. to (Et₄N)₂B₉H₉, (Et₄N)₂B₁₀H₁₀, Et₄NB₁₁H₁₄ and (Et₄N)₂B₁₂H₁₂ which are formed in varying proportions during the pyrolysis. A 1:1 Et₄NBH₄Et₃NBH₃ mixture gives the same mixture of final products in the same proportions as Et₄NBH₄ alone, but the reaction time is shorter.Results obtained under various conditions, for instance without solvent at 10⁻² torr (50% yield), are explained by the transfer of BH₃ groups occurring not only through Et₃NBH₃, but also by solid—solid reactions involving Et₄NBH₄. A more complete reaction of Et₃NBH₃ is obtained, giving quantitative yields, only when Et₃N is evacuated from the reaction mixture. Optimum conditions for the formation of each hydroborate are examined.     

Preparation of mono- or di-metal indenyl-iridium edrivatives and of tri-metal iridium-platinum complexes

Treatment of [IrCl(C₂H₄)₄] with K(C₉H₇) (C₉H₇ =indenyl) gives [Ir(C₂H₄)₂(η-C₉H₇)]. This compound is converted quantitatively into [Ir(CO)₂(η-C₉H₇)] by treatment with carbon monoxide. By reacting together these two iridium complexes [Ir₂(μ-CO)(CO)₂(ηC₉H₇)₂] has been obtained. The compound [Ir(CO)₂(η-C₉H₇)] reacts with [Pt(C₂H₄)₂{P(cyclo-C₆H₁₁)₃}] to give the complex [Ir₂Pt(CO)₃{P(cyclo-C₆H₁₁)₃}(η-C₉H₇)₂]. Protonation of the latter affords the salt [Ir₂Pt(μ-H)(CO)₃{P(cyclo-C₆H₁₁)₃}(μ-C₉H₇)₂] [BF₄]. The main features of the molecular structure of these complexes have been established by IR and NMR spectroscopy.     

Preparation of benzophenone imine complexes of transition metals

Benzophenone imine [M(η¹-NHCPh₂)(CO)_nP_5-n]BPh₄ [M = Mn, Re; n = 2, 3; P = P(OEt)₃, PPh(OEt)₂, PPh₂OEt, PPh₃] complexes were prepared by allowing triflate M(κ¹-OTf)(CO)_nP_5-n compounds to react with an excess of the imine. Hydride-imine [MH(η¹-NHCPh₂)P₄]BPh₄ (M = Ru, Os), triflate-imine [Os(κ¹-OTf)(η¹-NHCPh₂)P₄]BPh₄ and bis(imine) [Ru(η¹-NHCPh₂)₂P₄](BPh₄)₂ [P = P(OEt)₃] derivatives were also prepared. The complexes were characterized spectroscopically (IR, ¹H, ³¹P, ¹³C NMR) and a geometry in solution was also established. Hydride-benzophenone imine [IrHCl(η¹-NHCPh₂)L(PPh₃)₂]BPh₄and [IrHCl(η¹-NHCPh₂)L(AsPh₃)₂]BPh₄ [L = P(OEt)₃ and PPh(OEt)₂] complexes were prepared by reacting hydride IrHCl₂L(PPh₃)₂ and IrHCl₂L(AsPh₃)₂ precursors with an excess of imine. Dihydride IrH₂(η¹-NHCPh₂)(PPh₃)₃ complex was also obtained and a geometry in solution was proposed.     

Receptor of the serpentine-type and heterotrimeric G protein as targets of action of polylysine dendrimers

Molecular processes of the action of polycationic peptides that represent polylysine homo- and heterodendrimers on the functional activity of the biogenic amine- and peptide hormone-sensitive adenylyl cyclase signaling system (AC system) in rat myocardium and brains were studied. An intended use of these peptides is that of highly effective polymer carriers for biologically active substances. The polylysine homodendrimers of the third [(NH₂)₁₆(Lys)₈(Lys)₄(Lys)₂Lys-Ala-NH₂] (I), fourth [(NH₂)₃₂(Lys)₁₆(Lys)₈(Lys)₄(Lys)₂Lys-Ala-NH₂] (II), and fifth [(NH₂)₆₄(Lys)₃₂(Lys)₁₆(Lys)₈(Lys)₄(Lys)₂Lys-Ala-NH₂] (III) generations, as well as polylysine heterodendrimers of the fifth generation, [(NH₂)₆₄(Lys-Glu)₃₂(Lys-Glu)₁₆(Lys-Glu)₈(Lys-Glu)₄(Lys-Glu)₂Lys-Ala-Ala-Lys(ClAc)-Ala-NH₂] (IV), [(NH₂)₆₄(Lys-Ala)₃₂(Lys-Ala)₁₆(Lys-Ala)₈(Lys-Ala)₄(Lys-Ala)₂Lys-Ala-Lys(ClAc)-Ala-Ala-NH₂] (V) and [(NH₂)₆₄(Lys-Gly-Gly)₃₂(Lys-Gly-Gly)₁₆(Lys-Gly-Gly)₈(Lys-Gly-Gly)₄(Lys-Gly-Gly)₂Lys-Gly-Gly-Lys(ClAc)-Ala-Ala-NH₂] (VI), interact with the C-terminal regions of α subunits of the heterotrimeric G proteins, preferably of the inhibitor type, and stimulate its activity in respector-independent manner. The most effective G-protein activators were homodendrimers II and III and heterodendrimer V. The polylysine dendrimers disturbed the functional coupling of receptors of biogenic amines and peptide hormones with G_i proteins and, to a lesser extent, G_s proteins. This was manifested as a decrease in the regulatory effects of the hormones on AC activity and the GTP binding of the G protein, as well as by a decrease in the affinity of receptors to agonists in the presence of polylysine dendrimers, which is a consequence of the dissociation of the receptor-G protein complex. It has also been shown that, based on their molecular mechanisms and selectivity of action on G proteins, polylysine dendrimers are similar to mastoparan and melittin, which are natural toxins of insect venom.     

Specificity of the interaction of DNA-platinum, amount of platinum, and pH measurement]

Interaction between the sodium salt of a DNA extracted from salmon sperm (41% GC) with [Pt(NH₃)₄]Cl₂, [Pt(NH₂? (CH₂)₂? NH? (CH₂)₂? NH₂Cl]Cl, cis-Pt(NH₂? (CH₂)₂? NH₂)Cl₂, cis-Pt(NH₃)₂Cl₂, trans-Pt(NH₃)₂Cl₂, K[Pt(C₂H₄)Cl₃], and K₂[PtCl₄) indicates at least three types of complexation. A correlation is found between the change of pH and the number of platinum atoms fixed per (AT + GC) unit. The first binding site is located on the G-C pairs (guanine–cytosine), most likely the N-7(G) site, as it was shown in a previous study of the guanosine-platinum salts. The fixation of the second platinum atom by the pair (AT + GC) takes place with liberation of protons. In the case of the complexes cis-Pt(NH₂? (CH₂)₂? NH₂)Cl₂, cis-Pt(NH₃)₂Cl₂, and trans-Pt(NH₃)₂Cl₂ the second interaction seems to involve simultaneously the N-7(A) and the N-1(G) and N-3(C) sites. This latter intercrosslink between guanine and cytosine obviously liberates protons and the decrease of pH is related in this case to the trans effect of the platinum compounds. The first two platinum atoms in the reaction of K₂PtCl₄] or the Zeise salt, K[Pt(C₂H₄)Cl₃] with DNA are fixed on the G-C pairs. A maximum of six platinum atoms per (AT + GC) unit were fixed in this case. Preliminary experiments with a DNA extracted from bacteria Micrococcus lysodeikticus (72% GC) give similar results.     

Composition of leaf epicuticular waxes of Pteridium subspecies

The leaf epicuticular waxes of two subspecies of Pteridium consisted principally of alkyl esters (92 %; C₄₀–C₅₀) together with small amounts of n-alkanols (2 %; C₂₄–C₃₂) and hydrocarbons (2%; C₂₇–C₃₁). The esters comprised C₂₂–C₃₂ alkanols randomly combined with C₂₀ – C₂₄ fatty acids.     

Organic derivatives of aluminium. Part I. Reactions of alkanolamines with aluminium isopropoxide

Reactions of alkanolamines [R₁R₂NXOH; R₁ = H, CH₃, C₂H₅; R₂ = H, CH₃, C₂H₅ and X = -CH₂CH₂-, -CH₂CH₂CH₂-, -CH₂CHCH₃, -C₆H₄CH₂CH₂-] with aluminium isopropoxide in different molar ratios (1 to 3) yield compounds of the type Al(OPrⁱ)_3?n(OXNR₁R₂)_n, where ‘n’ can be 1, 2 and 3. Most of the derivatives are distillable liquids, soluble in common organic solvents and susceptible to hydrolysis even by atmospheric moisture. The new derivatives are characterized by elemental analysis, IR and ¹H NMR spectra. Molecular weight measurements of Al(OPrⁱ)_3?n(OXNR₁R₂)_n reveal them to be tetrameric in nature.     

Modeling aspects of hydrodesulfurization by molybdenum hydride compounds: Desulfurization of thiophene and benzothiophene and C-S bond cleavage of dibenzothiophene

The molybdenum hydride complexes Mo(PMe₃)₅H₂ and Mo(PMe₃)₄H₄ are capable of cleaving the C-S bonds of thiophene, benzothiophene and dibenzothiophene. For example, Mo(PMe₃)₅H₂ reacts with thiophene to give the η⁵-thiophene and butadiene-thiolate complexes, (η⁵-C₄H₄S)Mo(PMe₃)₃ and (η⁵-C₄H₅S)Mo(PMe₃)₂(η²-CH₂PMe₂). These complexes are also obtained from the reaction between Mo(PMe₃)₄H₄ and thiophene under photochemical conditions, whereas at elevated temperatures thiophene is desulfurized to liberate but-1-ene. Similarly, Mo(PMe₃)₄H₄ desulfurizes benzothiophene at elevated temperatures to liberate ethylbenzene, while the arylthiolate complex Mo(PMe₃)₄(SC₆H₄Et)H₃ is obtained photochemically. Furthermore, Mo(PMe₃)₄H₄ cleaves the C-S bond of dibenzothiophene to give [η⁶,κ¹-C₆H₅C₆H₄S]Mo(PMe₃)₂H.     

Characterization of ribonucleoprotein subparticles from 50 S ribosomal subunits of Escherichia coli.

Large ribonucleoprotein subparticles were recovered upon ribonuclease digestion of the 50 S ribosomal subunits of Escherichia coli, partially deproteinized by LiCl. Both their RNA and their protein compositions were analysed. The subunits, treated with LiCl at a concentration of 5.5 m, released an homogeneous subparticle containing proteins L₃, L₄, L₁₃, L₁₇, L₂₂ and L₂₉, about 70% of the 13 S fragment of 23 S RNA and about 50% of the 18 S one. Slightly larger species of subparticles were obtained from 50 S subunits treated with LiCl at concentrations between 3 m and 5 m; they contained in addition proteins L₂₀, L₂₁ and L₂₃ or L₂, L₁₄, L₂₀, L₂₁ and L₂₃ and a few small 23 S RNA fragments. No large subparticle was recovered from the 6 m-LiCl-treated 50 S subunits which contain only proteins L₃, L₁₃ and L₁₇. These LiCl subparticles were compared with those obtained from intact, unfolded and sodium doecyl sulphatetreated 50 S subunits.These studies reveal that in the presence of 0.10 m-magnesium acetate there is a very compact area within 50 S subunits consisting of proteins L₃, L₄, L₁₃, L₁₇, L₂₂ and L₂₉ and of about 60% of 23 S RNA; this area probably has an essential structural role. The results also show that 23 S RNA has a more folded conformation when within the 50 S subunit than when isolated, this conformation being stabilized by some of the 50 S proteins, in particular proteins L₄, L₂₂, L₂₀ and L₂₁. Finally these data permit a more definite localization of the primary and/or secondary binding sites of proteins L₂, L₃, L₄, L₁₄, L₁₇, L₂₀, L₂₁ and L₂₂ on 23 S RNA.     

Assay of molybdenum cofactor of barley

Conditions for assay of molybdenum cofactor in barley shoot extracts in the presence of molybdate (25 mM N₂MoO₄) and the sulphydryl-group protector, reduced glutathione (5 mM) were optimized. Both total Mo-cofactor (assayed after heat-treatment of cell-free extracts) and ‘free’ Mo-cofactor (assayed in untreated cell-free extracts) were assayed. Compared to control plants grown in the absence of an exogenous nitrogen source total Mo-cofactor levels increased around 70 % when plants were grown for 4 days in the presence of either 15 mM KNO₃ or 15 mM NH₄NO₃. Growth in the presence of 15 mM (NH₄)₂SO₄ did not affect the Mo-cofactor level. Very similar results were seen when plants were transferred to these nitrogen sources for 24 hr after previous growth in the absence of an exogenous nitrogen source. In contrast ‘free’ Mo-cofactor levels of both KNO₃ and NH₄NO₃-treated plants were increased 2-3-fold over untreated controls. Growth in the presence of (NH₄)₂SO₄ did not affect the ‘free’ Mo-cofactor level.