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采用一种新的重组方法,将来自集胞藻6803(Synechocystis sp PCC6803)的光系统I反应中心功能重组到脂质体中。

Functional reconstitution of photosystem I reaction center from cyanobacterium Synechocystis sp PCC6803 into liposomes using a new reconstitution procedure.

作者信息

Cladera J, Rigaud J L, Bottin H, Duñach M

机构信息

Department de Bioquímica i Biologia Molecular, Universitat Autonoma de Barcelona, Bellaterra, Spain.

出版信息

J Bioenerg Biomembr. 1996 Dec;28(6):503-15. doi: 10.1007/BF02110440.

DOI:10.1007/BF02110440
PMID:8953382
Abstract

Photosystem I reaction center from the cyanobacterium Synechocystis sp PCC6803 was reconstituted into phosphatidylcholine/phosphatidic acid liposomes. Liposomes prepared by reversephase evaporation were treated with various amounts of different detergents and protein incorporation was analyzed at each step of the solubilization process. After detergent removal the activities of the resulting proteoliposomes were measured. The most efficient reconstitution was obtained by insertion of the protein complex into preformed liposomes destabilized by saturating amounts of octylglucoside. In the presence of N-methylphenazonium methosulfate and ascorbic acid, liposomes containing the reaction center catalyzed a light-dependent net H+ uptake as measured by the 9-aminoacridine fluorescence quenching and the pH meter. An important benefit of the new reconstitution procedure is that it produces a homogeneous population of large-size proteoliposomes with a low ionic permeability and with a majority inwardly directed H+ transport activity. In optimal conditions, a light-induced delta pH of about 1.8 units could be sustained at 20 degrees C in the presence of valinomycin. In the absence of valinomycin, a "back-pressure" effect of an electrical transmembrane potential decreased both the rate and the extent of the H+ transport. The reaction center was also co-reconstituted with F0F1 H(+)-ATPases from chloroplasts and from the thermophilic bacterium, PS3. The co-reconstituted system was shown to catalyze a light-dependent phosphorylation which could only be measured in the presence of a high concentration of PSI (low lipid/PSI ratios) while no delta pH could be detected.

摘要

来自集胞藻属PCC6803蓝细菌的光系统I反应中心被重组到磷脂酰胆碱/磷脂酸脂质体中。通过反相蒸发制备的脂质体用不同量的不同去污剂处理,并在溶解过程的每个步骤分析蛋白质掺入情况。去除去污剂后,测量所得蛋白脂质体的活性。最有效的重组是通过将蛋白质复合物插入由饱和量的辛基葡糖苷使其不稳定的预先形成的脂质体中实现的。在硫酸N-甲基吩嗪鎓和抗坏血酸存在下,含有反应中心的脂质体催化了依赖光的净H⁺摄取,这通过9-氨基吖啶荧光猝灭和pH计进行测量。新重组程序的一个重要优点是它产生了具有低离子渗透性且大多数具有向内定向H⁺转运活性的均匀大尺寸蛋白脂质体群体。在最佳条件下,在缬氨霉素存在下于20℃可维持约1.8单位的光诱导ΔpH。在没有缬氨霉素的情况下,跨膜电势的“背压”效应降低了H⁺转运的速率和程度。反应中心还与来自叶绿体和嗜热细菌PS3的F₀F₁ H⁺-ATP酶共同重组。共同重组的系统显示出催化依赖光的磷酸化作用,这只能在高浓度的PSI(低脂质/PSI比率)存在下测量,而未检测到ΔpH。

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