山莨菪碱对重组鼠脑(Na~++K~+)—ATP酶旋转运动的影响

本文采用饱和转移顺磁共振技术研究了山莨菪碱对重组鼠脑(Ba~++K~+)-ATP酶旋转运动的影响.从鼠脑纯化的(Na~++K~+)-ATP酶经马来酰亚胺自旋探针标记,再重组于大豆磷脂脂质体.结果表明,(Na~++K~+)-ATP酶旋转相关时间为6—12微秒左右,山莨菪碱加速重组后的(Na~++K~+)-ATP酶的旋转运动.Arrhcnius图示出在10℃左右出现—明显折点,关于山莨菪碱抑制重组(Na~++K~+)-ATP酶活性与增加酶蛋白的旋转运动的关系进行了讨论.     

山莨菪碱对重组鼠脑(Na~++K~+)—ATP酶旋转运动的影响

本文采用饱和转移顺磁共振技术研究了山莨菪碱对重组鼠脑(Ba~++K~+)-ATP酶旋转运动的影响.从鼠脑纯化的(Na~++K~+)-ATP酶经马来酰亚胺自旋探针标记,再重组于大豆磷脂脂质体.结果表明,(Na~++K~+)-ATP酶旋转相关时间为6—12微秒左右,山莨菪碱加速重组后的(Na~++K~+)-ATP酶的旋转运动.Arrhcnius图示出在10℃左右出现—明显折点,关于山莨菪碱抑制重组(Na~++K~+)-ATP酶活性与增加酶蛋白的旋转运动的关系进行了讨论.     

(Na~++K~+)—ATP酶与磷脂膜的相互作用

本文研究了不同磷脂对兔肾外髓质(Na~++K~+)-ATP酶活性的影响、结果表明,DOPC、PG重组活性最高,用DMPC重组导致酶失活,酸性磷脂有利于维持该酶活性.DSC及自旋标记ESR实验结果示出(Na~++K~+)-ATP酶有选择地与酸性磷脂相互作用.     

(Na~++K~+)—ATP酶与磷脂膜的相互作用

本文研究了不同磷脂对兔肾外髓质(Na~++K~+)-ATP酶活性的影响、结果表明,DOPC、PG重组活性最高,用DMPC重组导致酶失活,酸性磷脂有利于维持该酶活性.DSC及自旋标记ESR实验结果示出(Na~++K~+)-ATP酶有选择地与酸性磷脂相互作用.     

山莨若碱通过膜脂影响兔肾(Na~++K~+)-ATP酶的构象及活性

研究了山莨菪碱对处于不同脂双层的兔肾外髓质(Na~++K~+)-ATP酶活性的影响,结果表明山莨菪碱对(Na~++K~+)-ATP酶的抑制作用与该酶所处的脂环境密切相关,如对去脂后的酶活性无明显影响,而对重组于酸性磷脂脂质体的酶比对重组于中性磷脂脂质体的酶有更大的抑制作用。园二色性实验表明,山莨菪碱使带349个界面脂分子的(Na~++K~+)-ATP酶二级结构发生明显变化,而对带189个界面脂分子的酶无明显作用。另外利用差示量热扫描研究表明山莨菪碱对酸性磷脂和中性磷脂脂质体或脂酶体相变行为有不同的影响。     

山莨若碱通过膜脂影响兔肾(Na~++K~+)-ATP酶的构象及活性

研究了山莨菪碱对处于不同脂双层的兔肾外髓质(Na~++K~+)-ATP酶活性的影响,结果表明山莨菪碱对(Na~++K~+)-ATP酶的抑制作用与该酶所处的脂环境密切相关,如对去脂后的酶活性无明显影响,而对重组于酸性磷脂脂质体的酶比对重组于中性磷脂脂质体的酶有更大的抑制作用。园二色性实验表明,山莨菪碱使带349个界面脂分子的(Na~++K~+)-ATP酶二级结构发生明显变化,而对带189个界面脂分子的酶无明显作用。另外利用差示量热扫描研究表明山莨菪碱对酸性磷脂和中性磷脂脂质体或脂酶体相变行为有不同的影响。     

羟基自由基对兔脑微粒体膜脂及膜蛋白的损伤

本文研究了过氧化氢与亚铁离子体系产生的羟基自由基对兔脑微粒体脂质过氧化作用及对膜上(Na~++K~+)-ATP酶活性的影响.结果表明,羟基自由基导致兔脑微粒体脂质过氧化,增加丙二醛的含量.羟基自由基还使微粒体膜巯基数下降,(Na~++K~+)-ATP酶活力受到抑制.阿魏酸钠对抑制微粒体脂质过氧化及对膜巯基和(Na~++K~+)-ATP酶均有保护作用.自旋捕集实验结果进一步证明药物对羟基自由基的猝灭作用.     

棉酚抑制(Na~++k~+)-ATP酶

 <正> 棉酚是一种效力很强的非甾体男用节育药。在口服棉酚的成年男性受试者中,在服药期间的不定阶段,有个别出现低血钾及肾性失钾的情况。由于细胞膜(Na~++K~+)-ATP酶是负责细胞内、外之间Na~+、K~+主动性转运的,故推测棉酚的这一毒副作用可能是它抑制跨细胞膜(特别是肾小管细胞)存在的(Na~++K~+)-ATP酶的结果。     

关于溴氰菊酯神经毒作用的生物化学研究

 本文利用生物化学的手段,对大鼠进行了急性和亚急性毒性实验,研究溴氰菊酯对动物中枢神经系统离子调节作用的影响。急性实验结果表明:<1>溴氰菊酯能显著抑制脑微粒体上的Ca~(2+)+Mg~(2+)-ATP酶和Na~++K~+-ATP酶活性,但并不降低ecto-Ca~(2+)-ATP酶(细胞表面的Ca~(2+)-ATP酶)的活性;<2>溴氰菊酯对大鼠小脑组织中的环腺苷酸含量无明显影响,但却能显著升高与其作用相反的环鸟苷酸含量。体外实验证明,溴氰菊酯能够减少线粒体对Ca~(2+)的主动摄取。在对大鼠进行的亚急性实验中,发现溴氰菊酯中毒组与对照组大鼠的Ca~(2+)+Mg~(2+)-ATP酶、Na~++K~+-ATP酶和ecto-Ca~(2+)-ATP酶的活性均无显著性差异。根据以上结果推测,在急性中毒的条件下,溴氰萄酯能引起大鼠脑神经细胞内Ca~(2+)和Na~+的浓度增高,致使神经兴奋性发生改变。     

菝葜皂甙原对Na~ 、K~ -ATP酶抑制的动力学研究

本文对菝葜皂甙原抑制Na~ 、K~ -ATP酶的动力学与机理进行了研究,并且与哇巴因的抑制作用进行了比较。动力学研究表明菝葜皂甙原抑制Na~ 、K~ -ATP酶,对底物Na~ 、K~ 均为混合性抑制剂;而对ATP则为反竞争性抑制剂。观察了磷脂对哇巴因和菝葜皂甙原抑制Na~ 、K~ -ATP酶的影响。磷脂不影响哇巴因的抑制作用;但多种磷脂都不同程度地降低菝葜皂甙原对Na~ 、K~ -ATP酶的抑制作用。     

Reconstitution of (Na+ + K+)-ATPase proteoliposomes having the same turnover rate as the membranous enzyme

Membranous (Na+ + K+)-ATPase from the electric eel was solubilized with 3-[3-cholamidopropyl)-dimethylammonio)-1-propanesulfonate (Chaps). 50 to 70% of the solubilized enzyme was reconstituted in egg phospholipid liposomes containing cholesterol by using Chaps. The obtained proteoliposomes consisted of large vesicles with a diameter of 134 +/- 24 nm as the major component, and their protein/lipid ratio was 1.25 +/- 0.07 g protein/mol phospholipid. The intravesicular volume of these proteoliposomes is too small to consistently sustain the intravesicular concentrations of ligands, especially K+, during the assay. The decrease in K+ concentration was cancelled by the addition of 20 microM valinomycin in the assay medium. The low value of the protein/lipid ratio suggests that these proteoliposomes contain one Na+/K+-pump particle with a molecular mass of 280 kDa per one vesicle as the major component. In these proteoliposomes, the specific activity of the (Na+ + K+)-ATPase reaction was 10 mumol Pi/mg protein per min, and the turnover rate of the ATP-hydrolysis was 3500 min-1, the same as the original enzyme under the same assay condition. The ratio of transported Na+ to hydrolyzed ATP was 3, the same as that in the red cell. The proteoliposomes could be disintegrated by 40-50 mM Chaps without any significant inactivation. This disintegration of proteoliposomes nearly tripled the ATPase activity compared to the original ones and doubled the specific ATPase activity compared to the membranous enzyme, but the turnover rate was the same as the original proteoliposomes and the membranous enzyme. This disintegration of proteoliposomes by Chaps suggests the selective incorporation of the (Na+ + K+)-ATPase particle into the liposomes and the asymmetric orientation of the (Na+ + K+)-ATPase particle in the vesicle.     

不同磷脂和糖脂对莱氏衣原体膜上Mg~（2＋）－ATPase活性的影响

莱氏衣原体膜上Ｍｇ~（２＋）－ＡＴＰａｓｅ用ＤＯＣ溶解后,经Ｓｅｐｈａｒｏｓｅ－６Ｂ和ＤＥＡＥ－ＣｅｌｌｕｌｏｓｅＤＥ－５２离子交换柱,得到了部分纯化的Ｍｇ~（２＋）ＡＴＰａｓｅ,并将此ＡＴＰａｓｅ与不同极性头部的磷脂和膜糖脂重组,研究了不同的极性头部的磷脂和膜糖脂对ＡＴＰａｓｅ活性的影响。此酶的活性不依赖酸性磷脂,ＰＧ、ＤＰＧ、大豆磷脂等明显抑制酶活性,中性磷脂ＤＭＰＣ、ＰＥ、ＰＣ则能增加酶活性,其中尤以非双层脂ＰＥ的作用最为明显。从莱氏衣原体膜上提取的糖脂（ＭＧＤＧ,ＤＧＤＧ）单独和ＡＴＰａｓｅ重组时,酶活性增加并不明显,当ＭＧＤＧ和ＤＧＤＧ以等比例混合时,能大大地增加酶活性。这表明Ｍｇ~（２＋）－ＡＴＰａｓｅ的活性很大程度上与磷脂的表面电荷及磷脂的组成相关。     

Cytoskeleton elements mediate the inhibition of the (Na++K+)atpase activity by PKC in Rhodnius prolixus malpighian tubules during hyperosmotic shock

In a previous paper, we observed that the specific activity of (Na++K+)ATPase of the isolated Malpighian tubules from Rhodnius prolixus is inhibited by protein kinase C (PKC) during hyperosmotic shock [Arenstein et al., J Membr Biol 146:47-57 [1995]; Caruso-Neves et al., Z Naturforsch 53c:911-917 [1998]). In the present paper, we study the involvement of the cytoskeleton in this process using isolated Malpighian tubules of Rhodnius prolixus. We observed that pre-incubation of the Malpighian tubule cells in hyperosmotic media decreases the specific activity of (Na++K+)ATPase by 90%. This effect was completely reversed when colchicine, which disrupts microtubules, or cytochalasin B, an inhibitor of actin microfilament polymerization, were added to the media in a dose-dependent manner. The maximal reversion was obtained with colchicine 7.0 microM or cytochalasin B 5.0 microM. The simultaneous addition of sphingosine 50 ng/mL, an inhibitor of PKC, to 10 microM colchicine or 5 microM cytochalasin B, in hyperosmotic media, did not change the stimulatory effect of these drugs on the specific activity of (Na++K+)ATPase. On the other hand, the co-incubation of TPA 20 ng/mL, an activator of PKC, to colchicine or cytochalasin B within hyperosmotic media, abolished the stimulatory effect of these drugs on the specific activity of (Na++K+)ATPase to a similar extent as hyperosmotic shock. These results suggest that inhibition of the (Na++K+)ATPase of the isolated Malpighian tubules from Rhodnius prolixus by PKC during hyperosmotic shock is mediated by cytoskeletal elements.     

山莨菪碱对肌质网Ca~(2+)-ATPase活力和转运功能的影响

本文研究了山莨菪碱对肌质网Ca~(2 )-ATPase活力及转运功能的影响.对膜结合及分离纯化的Ca~(2 )-ATPase,体系中加入不同量的药物都对酶的活力及转运效率无明显影响.当将药物与肌质网或纯化的Ca~(2 )-ATPase预保温后,山莨菪碱则表现出在低浓度使酶激活,高浓度抑制酶的活力.但都导致SRCa~(2 )转运效率降低.对用保温,超声及去污剂透析三种不同方法重建的脂酶体,结果表明:山莨菪碱通过作用于膜脂后,在低浓度激活Ca~(2 )-ATPase、高浓度抑制酶的活力.比较药物对不同类型纯磷脂重建的脂酶体活性的影响发现:山莨菪碱对含有酸性磷脂的脂酶体Ca~(2 )-ATPase的作用较不含酸性磷脂的要大.     

Ouabain binding to phospholipid-dependent adenosine triphosphatase.

The role of phospholipid in the binding of ouabain to the (Na+ + K+)-dependent adenosine triphosphatase was studied. Enzyme preparations obtained from rabbit kidney were treated with Lubrol WX to remove the phospholipid component essential for ATPase activity. Reconstituted enzyme samples were prepared by the addition of phosphatidylserine and sedimentation of an enzymically active lipid-protein complex. The binding of ouabain to both kinds of preparations was measured under equilibrium conditions with the use of 3H-labelled ouabain and initial ouabain concentrations in the range 0.01-1 micrometer. The main findings were: (i) (Mg2+ + Pi) promoted binding of significant quantities of ouabain only to the reconstituted enzyme; (ii) the absence of added Na+, (Mg2+ + ATP) similarly promoted binding only to the reconstituted samples; (iii) the addition of Na+ in the presence of (Mg2+ + ATP) increased the amount of ouabain bound to the reconstituted enzyme when the ouabain concentration was below about 0.1 micrometer, but it had no effect when the ouabain concentration was about 1 micrometer; (iv) (Mg2+ + ATP) induced ouabain binding to the depleted enzyme only when Na+ was also added; (v) the amount of ouabain bound to both depleted and reconstituted enzymes was the same in the presence of (Mg2+ + ATP + Na+); (vi) the reconstituted enzyme appeared to have a greater affinity for Na+ than did the depleted enzyme.     

A transport model for the (Na+/K+)ATPase in liposomes including the (Na+/K+)-channel function

(Na+/K+)ATPase liposomes of various degrees of reconstitution are formed by varying the amount of phosphatidylcholine added to the soluble (Na+/K+)ATPase before vesicles are formed by cholate removal. In the presence of ATP, the reconstituted sodium pump effectuates (Na+/K+) antiport. In the absence of ATP, the reconstituted sodium pump forms a (Na+/K+) channel. The stable plateaus formed by (1) the active Na+ transport, (2) the active K+ transport, (3) the 'passive' Na+ flux, and (4) the 'passive' K+ flux are determined in the optimally and the partially reconstituted liposomes. The activities of all four vectorial functions vary in a tightly correlated fashion, suggesting that they are mediated by the same transport-active configuration of (Na+/K+)ATPase. A transport model which includes the active and the passive (Na+/K+) fluxes mediated by the sodium pump in liposomes is outlined.     

Role of negatively charged phospholipids in highly purified (Na+ + K+)-ATPase from rabbit kidney outer medulla studies on (Na+ + K+)-activated ATPase, XXXIX.

1. The requirement for specific polar head groups of phospholipids for activity of purified (Na+ + K+)ATPase from rabbit kidney outer medulla has been investigated. 2. Comparison of content and composition of phospholipids in microsomes and the purified enzyme indicates that purification leads to an increase in the phospholipid/protein ratio and in phosphatidylserine content. 3. The purified preparation contains 267 molecules phospholipid per molecule (Na+ + K+)-ATPase, viz. 95 phosphatidylcholine, 74 phosphatidylethanolamine, 48 spingomyelin, 35 phosphatidylserine and 15 phosphatidylinositol. 4. Complete conversion of phosphatidylserine into phosphatidylethanolamine by the enzyme phosphatidylserine decarboxylase has no effect on the (Na+ + K+)-ATPase activity of the purified preparation. 5. Complete hydrolysis of phosphatidylinositol by a phospholipase C from Staphylococcus aureus, which is specific for this phospholipid, has no effect on the (Na+ + K+)-ATPase activity. 6. Hydrolysis of 95% of the phosphatidylcholine and 60--70% of the spingomyelin and phosphatidylethanolamine by another phospholipase C (Clostridium welchii) lowers the (Na+ + K+)-ATPase activity by about 20%. 7. Combination of the phospholipid-converting enzymes has the same effect as can be calculated from the effects of the enzymes separately. Only complete conversion of both phosphatidylserine and phosphatidylinositol results in a loss of 44% of the (NA+ + K+)-ATPase activity and 36% of the potassium 4-nitrophenylphosphatase activity. 8. These experiments indicate that there is no absolute requirement for one of the polar head groups, although in the absence of negative charges the activity is lower than in their presence.