Ca~（2＋）与含β－桐酸磷脂脂质体的相互作用

通过测定含β－桐酸（β－ＥＳＡ）的双棕榈酰磷脂酰胆碱（ＤＰＰＣ）脂质体在加入Ｃａ（２＋）后浊度,粒度及内包荧光物释放的变化,研究了Ｃａ（２＋）与ＤＰＰＣ／β－ＥＳＡ脂质体的相互作用,结果表明,ＤＰＰＣ／β－ＥＳＡ脂质体是一类对外加Ｃａ（２＋）敏感的脂质体,Ｃａ（２＋）的作用首先是引起脂质体间的集聚然后使脂质体融合;此时加速脂质体内包荧光物的释放。     

Ca~（2＋）与含β－桐酸磷脂脂质体的相互作用

通过测定含β－桐酸（β－ＥＳＡ）的双棕榈酰磷脂酰胆碱（ＤＰＰＣ）脂质体在加入Ｃａ（２＋）后浊度,粒度及内包荧光物释放的变化,研究了Ｃａ（２＋）与ＤＰＰＣ／β－ＥＳＡ脂质体的相互作用,结果表明,ＤＰＰＣ／β－ＥＳＡ脂质体是一类对外加Ｃａ（２＋）敏感的脂质体,Ｃａ（２＋）的作用首先是引起脂质体间的集聚然后使脂质体融合;此时加速脂质体内包荧光物的释放。     

Mn~(2+)对双棕榈酰磷脂酰胆碱——β-桐酸脂质体的~1H NMR谱的影响

本文研究了Mn~(2+)对双棕榈酰磷脂酰胆碱(DPPC)—β—桐酸(β-ESA—D_2O脂质体的~1HNMR谱的影响.当Mn~(2+)被加于DPPC-β-ESA-D_2O脂质体的外水相时,处于脂质体外表面和内表面的DPPC分子的-N~+(CH_3)_3的~1H NMR峰全都消失.当Mn~(2+)被加于DPPC—D_2O和DPPC—β—ESA—D_2O混合脂质体的外水相时,所有的-N(CH_3)_3的~1H NMR峰也都消失.这个现象被认为是β-ESA与Mn~(2+)相结合及其在脂质体的里.外分子层间和在脂质体间转移的结果.     

表面活性剂TritonX－100对菌紫质蛋白紫外荧光性质的影响

用荧光光谱方法研究了ＴｒｉｔｏｎＸ－１００（以下缩写为ＴＸ－１００）对菌紫质蛋白（Ｂａｃｔｅｒｉｏｒｈｏｄｏｐｓｉｎ,ＢＲ）及视黄醛生色团漂白后的紫膜（Ｂａｔｅｒｉｏｐｓｉｎ,ＢＯ）紫外荧光性质的影响．结果表明：表面活性剂ＴＸ－１００使ＢＲ中色氨酸在３２６ｎｍ处的荧光发射强度增加。随着ＴＸ－１００对ＢＲ的增溶,改变了生色团的构象环境,破坏了ＢＲ中色氨酸与生色团之间的能量转移。增溶后的ＢＲ中,Ｔｒｐ趋向于更疏水性的环境。     

三价盐对C_8-卵磷脂胶团溶液相分离的作用

用激光散射技术结合浊点法测定了加有不同离子强度的四种三价稀土盐（ＬａＣｌ３,ＣｅＣｌ３,Ｌａ（ＮＯ３）３,Ｃｅ（ＮＯ３）３）的Ｃ８－卵磷脂溶液的液－液相分离曲线,从中得出了相分离临界温度（Ｔｃ）和临界浓度（Ｘｃ）随盐类型和盐离子强度变化曲线。发现各种三价盐都使Ｔｃ和Ｘｃ随离子强度的增加先降低,然后再使之升高。其变化也遵循我们导出的式子：ＴＣ＝ＴＣ０＋Ａ１Ｉ１２－Ａ２Ｉ所描述的规律。各种正、负离子对Ｔｃ和Ｘｃ的相对作用程度分别为：Ｃｅ３＋＞Ｌａ３＋;ＮＯ３－＞Ｃｌ－。用液－液相分离曲线的实验数据,根据吉布斯自由能模型,还计算了胶团的作用因子Ｃ和形成因子Δμ．借助这两个表象参数,利用加盐表面活性物胶团溶液的唯象理论,从理论上算出了各两相共存曲线,其结果与实验值的吻合令人满意。     

大豆卵磷脂对小鼠的抗疲劳和抗氧化作用研究

目的:研究大豆卵磷脂的抗疲劳及抗氧化作用。方法:小鼠经口给予大豆卵磷脂30天后,采用负重游泳实验,观察记录小鼠游泳死亡时间;检测血清尿素氮、肝糖原;测定血清和肝匀浆超氧化物歧化酶(SOD)活性、谷胱甘肽过氧化物酶(GSH-Px)活力、丙二醛(MDA)含量。结果:给予大豆卵磷脂后,与对照组相比,实验组小鼠负重游泳时间明显延长,肝糖原消耗量减少,降低运动后血清尿素氮水平(P<0.05);升高小鼠血清和肝匀浆SOD活性及GSH-Px活力,降低MDA的含量(P<0.05)。结论:大豆卵磷脂具有抗疲劳和抗氧化作用。     

大豆卵磷脂对小鼠的抗疲劳和抗氧化作用研究

目的：研究大豆卵磷脂的抗疲劳及抗氧化作用。方法：小鼠经口给予大豆卵磷脂30天后,采用负重游泳实验,观察记录小鼠游泳死亡时间;检测血清尿素氮、肝糖原;测定血清和肝匀浆超氧化物歧化酶（SOD）活性、谷胱甘肽过氧化物酶（GSH—Px）活力、丙二醛（MDA）含量。结果：给予大豆卵磷脂后,与对照组相比,实验组小鼠负重游泳时间明显延长,肝糖原消耗量减少,降低运动后血清尿素氮水平（P〈0．05）;升高小鼠血清和肝匀浆SOD活性及GSH-Px活力,降低MDA的含量（P〈0．05）。结论：大豆卵磷脂具有抗疲劳和抗氧化作用。     

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.     

对盐和C_8-卵磷脂水溶液的准弹性激光散射研究

本文用自差拍光混频的准弹性激光散射技术,对生物组织重要组成部分的C_a-卵磷脂水溶液内微团的流体力学半径随卵磷脂浓度,温度,添加的单价盐离子类型和强度的变化情况,进行了系统性研究.并根据微团形成的梯级模型,推导出微团的大小和结构在微团形成过程中的变化,微团形成参数以及盐控制微团形成的规律.     

铝离子对二价铁离子启动的卵磷脂脂质体脂质过氧化的影响

利用化学发光、ＴＢＡ 反应与测量共轭二烯的方法观测了Ａｌ３ ＋ 对Ｆｅ２ ＋ 启动的卵磷脂脂质体脂质过氧化的影响。实验结果显示,在生理ｐＨ 条件下,Ａｌ３ ＋ 对Ｆｅ２ ＋ 启动的脂质过氧化有增强作用,表现为缩短潜伏期和加快脂质过氧化的反应速率, Ａｌ３ ＋ 的增强作用与脂质体中原先存在的过氧化物有关。这可能是因为在脂质体存在的条件下,Ａｌ３ ＋ 加速了Ｆｅ２ ＋ 的氧化,且加速作用与脂质体中原先存在的过氧化物的含量有关;另一方面,Ａｌ３ ＋ 可以引起脂质体的聚集,表现为浊度的增加;测量脂质体上标记的脂肪酸自旋标记物５ － Ｄｏｘｙｌ ｓｔｅａｒｉｃ ａｃｉｄ 的ＥＳＲ 波谱发现： Ａｌ３ ＋ 降低了脂质体的膜脂的流动性。研究表明： Ａｌ３ ＋ 对Ｆｅ２ ＋ 启动的卵磷脂脂质体的过氧化的增强作用可能与Ａｌ３ ＋ 加速了Ｆｅ２ ＋ 的氧化和改变了脂质体的物理状态有关     

Triton X－100对紫膜蛋白的效应

本文采用同步辐射小角Ｘ射线散射方法研究了用非离子表面活性剂ＴｒｉｔｏｎＸ—１００处理后的嗜盐菌紫膜及其视紫红质蛋白结构的变化。实验结果表明,用不同浓度的ＴｒｉｔｏｎＸ—１００处理紫膜碎片时,紫膜及其蛋白所处的状态有着很大变化。     

Triton X-100对细菌视紫红质中间产物M_(412)的效应

本文研究用非离子表面活性剂Triton X-100处理后的细菌视紫红质(BR Bacteriorhodo-psin)光循环中间产物M_(412)动力学过程的变化.实验结果表明,用不同浓度的Triton处理pH=6.5的BR体系时,其中间产物M_(412).快衰减成分的半衰期(τ_(1/2)~f)在Triton浓度为0.05%(w/w)附近突然变慢,随着Triton浓度的加大,τ_(1/2)~f又逐渐加快;慢衰减部分的半衰期(τ_(1/2)~s)则随Tri-ton浓度的增加逐渐变慢.BR的生色团峰发生蓝移.说明不同浓度的Triton在水溶液中聚集状态不同,可不同程度地破坏膜脂的液晶态结构,从而导致镶嵌在其中的BR发生构象的变化,使转运质子的氢键通道受到不同程度的影响,故质子泵转运通道发生改变、致使M_(412)的衰减速率改变.     

THE SUBCELLULAR LOCALIZATION OF Ach SYNTHESIS IN RAT STRIATAL SYNAPTOSOMES INVESTIGATED WITH THE USE OF TRITON X-100

—The regulation of [¹⁴C]ACh synthesis was studied in rat striatal synaptosomes incubated in presence of various concentrations of Triton X-100, using [2-¹⁴C]pyruvate or [6-¹⁴C]glucose as precursors. The progressive rupture of the cytoplasmic and mitochondrial compartments induced by the non-ionic detergent was followed by studying the release, into the incubating medium, of lactate dehydrogenase and choline acetyltransferase (ChAc) and of fumarate hydratase, respectively. [³H]Choline uptake (1 μm ) was measured to determine the activity of the high affinity choline permease. ¹⁴CO₂ formation from [2-¹⁴C]pyruvate was used as an index of the Krebs cycle activity. The rate of [¹⁴C]ACh synthesis from [2-¹⁴C] pyruvate was dependent on the Triton X-100 concentration; the ester formation decreased between 0·001% (v/v) and 0·010%, but increased again beyond this concentration of detergent. This last phenomenon was interpreted as the result of an extracellular synthesis of ACh involving pyruvate dehydrogenase and ChAc. At 0·002% Triton X-100 the ¹⁴CO₂ formation was not affected, indicating a normal mitochondrial activity. The decrease of [¹⁴C]ACh synthesis observed up to this detergent concentration could be correlated to the decline of the highaffinity choline permease activity. In these experimental conditions, the ester synthesis could not be restored by the addition of large amounts of choline in the incubating medium suggesting that the molecules of choline must cross the high-affinity choline permease system in order to be acetylated. This could indicate a close association between the permease and choline acetyltransferase.     

ACTION OF TRITON X-100 ON CHLOROPLAST MEMBRANES : Mechanisms of Structural and Functional Disruption

Addition of Triton X-100 to chloroplast suspensions to a final concentration of 100–200 µM causes an approximate tripling of chloroplast volume and complete inhibition of light-induced conformational changes, light-dependent hydrogen ion transport, and photophosphorylation. Electron microscopic studies show that chloroplasts treated in this manner manifest extensive swelling in the form of vesicles within their inner membrane structure. Triton was adsorbed to chloroplast membranes in a manner suggesting a partition between the membrane phase and the suspending medium, rather than a strong, irreversible binding. This adsorption results in the production of pores through which ions may freely pass, and it is suggested that the inhibition of conformational changes, hydrogen ion transport, and photophosphorylation by Triton is due to an inability of treated chloroplast membranes to maintain a light-dependent pH gradient. The observed swelling is due to water influx in response to a fixed, osmotically active species within the chloroplasts, after ionic equilibrium has occurred. This is supported by the fact that chloroplasts will shrink upon Triton addition if a nonpenetrating, osmotically active material such as dextran or polyvinylpyrrolidone is present externally in sufficient concentration (>0.1 mM) to offset the osmotic activity of the internal species.     

二价金属离子对脂质体影响的激光拉曼光谱研究

本文运用激光拉曼光谱技术,在25℃测量温度下研究了Mg~(2 )、Mn~(2 )、Cu~(2 )对DPPC、DPPA、DOPC、DOPA脂质体及L(o)PC脂质微团磷脂碳氢链的构象及运动状态的影响。对实验数据的分析表明,在二价金属离子对膜脂的影响中,膜脂起了主导作用。对于相同极性头部的磷脂,二价金属离子影响的强弱取决于碳氢链的组分。即:当碳氢链为饱和脂肪酸时,二价金属离子能导致膜脂的物理状态发生较大的变化。当碳氢链为具有一个不饱和键的脂肪酸时,金属离子的影响较小。而且,在碳氨链侧向耦合较弱的情况下,金属离子的作用也相对较弱。     

用ESR自旋捕集法研究吸烟烟气处理的脂质体对大鼠粒细胞产生O_2~-的影响

吸烟烟气能引发卵磷脂脂质体的脂质过氧化。若将吸烟烟气处理20s的脂质体作用完整的大鼠粒细胞(RPN),用ESR自旋捕集方法发现,当作用时间在25min内(脂浓度1.0mg/ml)或脂浓度小于15.0mg/ml(而作用时间均为15min)时,这种过氧化的脂质体能增加RPN呼吸爆发产生O_2~-的量。而没有经吸烟烟气处理的新制脂质体,在脂浓度大于0.2mg/ml(作用时间15min)时,都不同程度地抑制RPN产生O_2~-。     

用ESR自旋捕集法研究吸烟烟气处理的脂质体对大鼠粒细胞产生O_2~-的影响

吸烟烟气能引发卵磷脂脂质体的脂质过氧化。若将吸烟烟气处理20s的脂质体作用完整的大鼠粒细胞(RPN),用ESR自旋捕集方法发现,当作用时间在25min内(脂浓度1.0mg/ml)或脂浓度小于15.0mg/ml(而作用时间均为15min)时,这种过氧化的脂质体能增加RPN呼吸爆发产生O_2~-的量。而没有经吸烟烟气处理的新制脂质体,在脂浓度大于0.2mg/ml(作用时间15min)时,都不同程度地抑制RPN产生O_2~-。     

电子自旋共振波谱技术研究不同pH值对二棕榈酰磷脂酸脂质体相变性质的影响

本文用电子自旋共振(ESR)波谱技术研究了不同pH值对酸性磷脂二棕榈酰磷脂酸(DPPA)脂质体相变性质的影响。结果表明:DPPA脂质体随pH值的增加其相变温度降低。通过对测试条件的选择和波谱参数的测量,TEMPO标记的DPPA脂质体在HEPES溶液中ESR谱不出现疏水峰的原因,是由于仪器分辨率不够以及自旋标记探针TEMPO在DPPA脂质体脂双层疏水相中的超精细偶合常数Ao和各向同性go因子与它们在HEPES溶液中的值相近。     

THE DISSOCIATION OF RAT BRAIN MEMBRANES BEARING ACETYLCHOLINESTERASE BY THE NON-IONIC DETERGENT TRITON X-100 AND AN EXAMINATION OF THE PRODUCT

Abstract— The action of Triton X-100 on a membrane preparation from rat brain was studied with reference to the solubilization of acetylcholinesterase and the product was characterized by exclusion chromatography. The AChE and membrane protein were readily solubilized to form particles corresponding to a mol. wt. of about 5 × 10⁵. The solubility of these particles depended on the continued presence of the detergent. It was concluded that these soluble particles formed an intermediate stage in organization between membrane-bound AChE and the soluble protein enzyme, and perhaps represented preexisting lipoprotein subunits of the membranes.