膜融合剂对脂质体及血影膜膜流动性的影响

本文用荧光探针ANS,DPH与A研究了几种膜融合剂对脂质体与血影膜流动性的影响.蔗糖使PS脂质体的脂双层流动性降低,探针越是在极性区流动性越小,说明蔗糖主要作用于脂双层的极性区;蔗糖也使血影膜流动性降低,此作用是可逆的.油酸甘油脂(GMO)使PS脂质体的流动性增加,且越是在疏水区内部,流动性增加得越大,说明GMO主要是作用于脂双层的非极性区:GMO也使血影膜流动性增加,此作用是不可逆的.二甲亚砜(DMSO)对血影膜的作用,两种不同荧光探针不一样,对DPH的作用出现双相让,低浓度与高浓度的作用结果分别与蔗糖和GMO的作用一致.     

精胺对脂质体及细胞膜融合的作用

本文通过共振能量转移法与三氯化铽荧光法探讨了精胺及其与Ca~(2 )对脂质体及人红细胞膜融合的诱导作用.结果表明,精胺能诱导PS脂质体的凝聚,但不能诱导其融合.精胺能诱导血影膜的融合.精胺与Ca~(2 )一起使用.对脂质体及血影膜的融合都分别有协同增效作用.     

磷脂酶C诱导膜融合的初步研究

用光散射、电镜和荧光共振能量转移技术研究了ＰＬＣ诱导两种单一膜脂组分的模型膜即二油酸磷脂酰胆碱（ＤＯＰＣ：ｄｉｏｌｅｏｙｌｐｈａｐｈｅｔｉｄｙｌｃｈｏｌｉｎｅ）脂质体和二豆蔻酰磷脂酰胆碱（ＤＭＰＣ：ｄｉｍｙｒｉｓｔｏｙｌｐｈｏｐｈａｔｉｄｙｌｃｈｅｌｏｎｅ）脂质体膜融合的可能性。结果表明：ＰＬＣ可以引起ＤＯＰＣ脂质体的融合。在相同的条件下,未见到ＤＭＰＣ脂质体的融合。这就首次证明了ＰＬＣ诱导单一组分脂质体融合的可能性。结果还表明：ＰＬＣ诱导脂质体膜融合的可能性大小与膜脂结构有关。用大鼠血影膜、人红细胞膜、大鼠巨噬细胞膜和大花萱草花瓣原生质体膜等天然生物膜作为材料,研究了磷脂酶Ｃ（ＰＬＣ：ｐｂｏｓｐｈｏｌｉｐａｓｅＣ）诱导上述各种天然膜融合的可能性,均未观察到膜融合现象。提示ＰＬＣ不易诱导天然细胞膜的融合。     

稀土离子对带3蛋白阴离子转运活性及血影膜流动性的影响

测定了Ｌａ２＋、Ｇｄ３＋、Ｔｂ３＋及Ｙｂ３＋四种稀土离子对带３蛋白阴离子转运活性及对血影膜脂流动性的影响。结果如下：（１）稀土离子可强烈抑制带３蛋白的阴离子转运活性,抑制程度随稀土离子浓度增加而增加,最高达到６３．７％。（２）不同的稀土离子对带３蛋白的抑制程度不同,抑制程度从大到小的顺序为Ｙｂ＞Ｔｂ＞Ｇｄ＞Ｌａ。（３）稀土离子可显著降低血影膜流动性,并且在脂双层的全部厚度内都降低,降低的程度随稀土浓度的增大而增大。（４）不同的稀土离子对血影膜流动性的影响不同,作用从大到小的顺序与它们对带３蛋白活性抑制程度大小的顺序一致。（５）稀土离子对血影膜流动性的影响特征与稀土离子抑制带３蛋白活性的特征完全相符,带３蛋白中承担阴离子转运功能的部分是贯穿性膜蛋白,并且在阴离子转运过程中要发生显著的构象变化,因此稀土离子可能是通过作用于膜脂再影响带３蛋白活性的。     

融合膜中PSⅡ激发的电子推动嵴膜的电子传递和磷酸化

利用毛地黄苷从菠菜叶绿体类囊体膜制备了PSⅡ颗粒,氧化还原差示光谱及SDS-聚丙烯酰胺凝胶电泳结果表明其具备PSⅡ的典型特征,它具有从水氧化到质醌还原的酶活性。从大豆磷脂用超声法制备了脂质体。从鼠肝线粒体分离了嵴膜。将制备的PSⅡ颗粒预组装于脂质体,然后将此预组装物(PSⅡ—PL)再与嵴膜组合,此膜系于光下获得了相当量的ATP合成,证明了融合膜中PSⅡ电子传递可推动嵴膜的电子传递和磷酸化机构合成ATP。     

毕氏海蓬子类囊体膜与卵磷脂重组脂质体的耐热性研究

采用卵磷脂(PC)构建脂质体,然后将毕氏海蓬子类囊体膜蛋白复合物重组到脂质体中.分析不同温度(25℃、35℃、45℃和55℃)处理后蛋白脂质体的电子传递活性、吸收光谱和荧光光谱的变化,以探讨膜脂与膜蛋白在高温胁迫下的交互作用.结果显示:蛋白脂质体光系统Ⅱ(PSⅡ)的放氧活性和光系统Ⅰ(PSⅠ)的耗氧活性随着PC比例的提高而增加,在PC与类囊体膜比例为4∶1(Lipid∶Chl,w/w)时达到最高,同时蛋白脂质体的吸收光谱和荧光光谱也呈上升趋势;在PC与类囊体膜重组比例为4∶1条件下,高温处理后的蛋白脂质体的PSⅡ放氧活性和PSⅠ耗氧活性显著大于未经重组的,其吸收光谱和荧光光谱峰值下降幅度低于未经重组的,且峰位基本没有变化.研究表明,PC可能通过增加结合天线的大小来促进蛋白脂质体对光能的吸收和能量从外周天线到PSⅡ和PSⅠ核心复合物的传递;在脂质体中,PC与类囊体膜的交互作用提高了PSⅡ和PSⅠ在高温胁迫下的光化学效率,增强了PSⅡ和PSⅠ的耐热性.     

竹红菌甲素对红细胞膜和几种磷脂脂质体膜的流动性的光敏损伤

本文以荧光探针为手段,通过测量膜偏振度的变化,探讨了竹红菌甲素光敏作用对红细胞膜和几种磷脂脂质体膜的流动性的损伤。结果表明,甲素光敏作用使不同种类的磷脂(DPPC,DPPC/DPPE,红细胞膜磷脂)脂质体的流动性增加,其对光敏作用的敏感程度为红细胞膜磷脂脂质体显著小于DPPC/DPPE脂质体及DPPC脂质体。对红细胞膜来说,甲素光敏作用使其流动性呈现先降低而后增加的现象。去除膜上的spectrin以及用胰蛋白酶处理可使这种流动性变化的幅度受到抑制。据此,我们认为,膜磷脂,膜蛋白对甲素光敏作用中膜流动性的变化有着不同的影响,膜蛋白,特别是spectrin,是其中极重要的因素。     

三氯乙烯对脂质体膜通透性的影响及其破膜效应

本文通过测定脂质体膜对水的通透性及脂质体对被包裹血红蛋白的释放率,研究了三氯乙烯对脂质体的作用.观察到在低浓度时,三氯乙烯能增加蛋卵磷脂脂质体的通透性,随着浓度的增加有破膜释放的效应.     

艾氏腹水癌细胞膜质子跨膜外转运与脂质体融合:Ca2+及脂质体膜脂成份的作用

研究了Ca^2 及脂质体膜脂成分对艾氏腹水癌细胞质膜质子跨膜转运驱动的脂质体融合中的作用。结果 表明Ca^2 促进质子跨膜转运驱动的质子跨膜转运驱动艾氏腹水癌细胞与脂质体间的融合,膜融合程度与膜表面电荷密度的相关曲线显示,在下述条件膜融合与膜表面电荷密度呈正相关：（1）介质Ca^2 浓度小于6mmol/L,脂质体磷脂组成为PE：PC：CL＝6：2：2;（2）介质Ca^2 浓度为6mmol/L,脂质体鳞脂组成为PE：PC：CL＝6：2：2;（3）无Ca^2 介质,脂质体磷脂组成为PE：CL＝8：2;（4）介质Ca^2 浓度10mmol/L,脂质体磷脂组成为PE：CL＝8：2。脂质体PE／PC含量对膜融合的影响表明,当PE含量减少PC含量增加时,膜融合程度不断下降,提示影响膜融合的另一因素可能是生物膜结构形成“柄”融合中介体的能力。     

用脂肪酸自旋标记研究库存血红细胞膜的流动性

用两种脂肪酸自旋标记物5—DOXYL和16-DOXYL研究了ACD-B库存血保存期间红细胞膜的流动性及其温度相关性.结果发现:血液保存期间红细胞膜浅层流动性降低,深层流动性增高;红细胞膜浅层相变温度点明显降低,红细胞膜深层则出现两个相变温度点T_1和T_2在血液保存期间T_1和T_2逐渐接近并最后融合成一个相变温度点.     

Fusion in phospholipid spherical membranes. II. Effect of cholesterol, divalent ions and pH.

Effect of cholesterol, divalent ions and pH on spherical bilayer membrane fusion was studied as a function of increasing temperature. Spherical bilayer membranes were composed of natural [phosphatidylcholine (PC) and phosphatidylserine (PS)] as well as synthetic (dipalmitoyl-PC, dimyristoyl-PC and dioleoyl-PC) phospholipids. Incorporation of cholesterol into the membrane (33% by weight) suppressed the fusion temperature and also greatly reduced the percentage of membrane fusion. The presence of 1 mM divalent ions (Ca++, Mg++ or Mn++) on both sides or one side of the PC membrane did not affect appreciably its fusion characteristic with temperature, but the PS membrane fusion with temperature was greatly enhanced by the presence of divalent ions. The variation of pH of the environmental solution in the range of 5.5 approximately 7.0 did not affect the membrane fusion characteristic. However, at pH 8.5, the fusion with respect to temperature was shifted toward the lower temperature by approximately 3degreesC for PC and PS membranes, and at pH 3.0 the opposite situation was observed as the fusion temperature was increased by 6degreesC for PS membranes and by 4degreesC for PC membranes The results seem to indicate that membrane fluidity and structural instability in the bilayer are important for membrane fusion to occur.     

Proteoliposome interaction with human erythrocyte membranes. Functional implantation of gamma-glutamyl transpeptidase

The transfer of detergent solubilized and purified gamma-glutamyl transpeptidase (gamma-GTase), of hog kidney cortex, from proteoliposomes into human erythrocyte ghost membranes has been studied. The transfer of gamma-glutamyl transpeptidase was observed upon incubation of gamma-GTase incorporated dipalmitoylphosphatidylcholine vesicles with erythrocyte ghost membranes at 37 degrees C for 12 h. The extent of transfer was dependent upon the fluidity of donor proteoliposomes, being more when dipalmitoylphosphatidylcholine proteoliposomes were used compared to dimyristoylphosphatidylcholine, and intermediate values were observed when binary mixtures of DMPC and DPPC were used. Moreover, the transfer of gamma-GTase was facilitated when rigid basic phospholipid proteoliposomes were used as donor. The transfer of gamma-GTase has been observed to be associated with the removal of intrinsic membrane proteins and lipids from erythrocytes, mainly acetylcholinesterase, sphingomyelin, and cholesterol. An enhancement in the fluorescence due to resonance energy transfer was observed when ghost membranes containing fluorescent donor probe were incubated with proteoliposomes containing fluorescent acceptor probe, indicating that fusion but not adsorption of vesicles occurs during the transfer process. However, the inability of entrapped [14C]-sucrose delivery from proteoliposomes into ghost membrane vesicle suggest that fusion per se is not primarily involved in the transfer process. It appears that the transfer of gamma-glutamyl transpeptidase occurs by a collisional transfer process resulting in intermembrane protein transfer. The gamma-glutamyl transpeptidase implanted ghost membranes exhibited the uptake of L-glutamate which was inhibited by serine-borate, an inhibitor of transpeptidase activity. In addition, the uptake of L-glutamate was inhibited by the dipeptide gamma-glutamyl-L-glutamate, thus supporting the proposed role of gamma-glutamyl transpeptidase in the uptake of amino acids in biological membranes.     

Interaction of human erythrocyte ghosts or liposomes with polyethylene glycol detected by fluorescence polarization

The membrane fluidity of human erythrocyte ghost was temporarily increased by the addition of polyethylene glycol with molecular weight of 7500. On the other hand, the fluidity of dipalmitoylphosphatidyl choline bilayer liposomes was monotonously decreased by the addition of polyethylene glycol. Fusion of liposomes was inhibited by the interaction with polyethylene glycol. The temporary increase in membrane fluidity of erythrocyte ghosts was considered to be the result of the clustering of membrane-bound proteins which is believed to be one of the most important sequences in cell fusion.     

Sendai virus-erythrocyte membrane interaction: quantitative and kinetic analysis of viral binding, dissociation, and fusion.

A kinetic and quantitative analysis of the binding and fusion of Sendai virus with erythrocyte membranes was performed by using a membrane fusion assay based on the relief of fluorescence self-quenching. At 37 degrees C, the process of virus association displayed a half time of 2.5 min; at 4 degrees C, the half time was 3.0 min. The fraction of the viral dose which became cell associated was independent of the incubation temperature and increased with increasing target membrane concentration. On the average, one erythrocyte ghost can accommodate ca. 1,200 Sendai virus particles. The stability of viral attachment was sensitive to a shift in temperature: a fraction of the virions (ca. 30%), attached at 4 degrees C, rapidly (half time, ca. 2.5 min) eluted from the cell surface at 37 degrees C, irrespective of the presence of free virus in the medium. The elution can be attributed to a spontaneous, temperature-induced release, rather than to viral neuraminidase activity. Competition experiments with nonlabeled virus revealed that viruses destined to fuse do not exchange with free particles in the medium but rather bind in a rapid and irreversible manner. The fusion rate of Sendai virus was affected by the density of the virus particles on the cell surface and became restrained when more than 170 virus particles were attached per ghost. In principle, all virus particles added displayed fusion activity. However, at high virus-to-ghost ratios, only a fraction actually fused, indicating that a limited number of fusion sites exist on the erythrocyte membrane. We estimate that ca. 180 virus particles maximally can fuse with one erythrocyte ghost.     

肺叶切除术对红细胞及淋巴细胞膜流动性的影响

目的：研究肺叶切除术对红细胞及淋巴细胞膜流坳性的影响。方法：选择２０例择期开胸手术病人,均作肺叶切除术。分别用微量滴定法、高效液权色谱法和ＤＰＨ荧光探剂法测定血浆和红细胞膜ＰＬＡ２活性,红细胞膜磷脂ＰＳ、ＰＥ、ＰＣ和红细胞、淋巴膜脂流动性。结果：手术１０ｍｉｎ、手术６０ｍｉｎ和手术结束后３０ｍｉｎ血浆和红细胞膜ＰＬＡ２活性均显著高于麻醉诱导前;手术６０ｍｉｎ和手术结束后３０ｍｉｎ 红细胞膜ＰＳ、Ｐ     

Effect of sealing on the incorporation of pyrene in goat erythrocyte ghosts — A fluorescence study

The incorporation of pyrene within the membrane interior of goat erythrocyte ghost has been estimated from its fluorescence spectrum. The excimer to monomer fluorescence intensity ratio of embedded pyrene is a function of the fluidity of its environment and the magnitude of its incorporation. Our study shows that this ratio is considerably less (30%) in a pre-sealed ghost than in the non-sealed ghost revealing that the site of incorporation of the probe is indeed the hydrophobic interior of the membrane; as in the later case, the probe has access to the membrane interior from both sides of the membrane. Our study on kinetics of molecular exchange indicates a very fast (of the order of seconds) transfer rate of pyrene from probed to unprobed erythrocyte ghosts through the aqueous phase rather than actual fusion of the membranes.     

没食子酸丙酯和没食子酸异丁酯对人红细胞膜结构与功能的影响

本文应用荧光探剂ANS(1—苯胺—8萘磺酸)、NPN(N—苯基—1—萘胺)和DPH(1.6—二苯基—1.3.5—已三烯)观察没食子酸丙醋和没食子酸异丁酯对人红细胞膜流动性和相变温度以及Na~ -K~ ATP酶活性的影响.实验结果指出该两种化合物均能:(1)降低与膜结合的荧光探剂强度但不改变探剂在水相与膜相的分配比例:(2)降低膜脂的相变温度,增加膜的流动性;(3)抑制红细胞膜Na~ -K~ ATP酶活性;(4)标记红细胞膜的DPH偏振度随化合物浓度的增加而降低,膜的流动性增加.在给定的浓度范围内,两种化合物的效应表现为明显的量效关系与构效关系.从上述结果推测该两种化合物可能是通过改变膜脂结构、膜蛋白的脂类环境而调节膜的功能,成为其治疗疾病的机理之一.