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将捕光复合物和光系统II核心重组到半乳糖脂和磷脂脂质体中。

Reconstitution of light-harvesting complexes and photosystem II cores into galactolipid and phospholipid liposomes.

作者信息

Sprague S G, Camm E L, Green B R, Staehelin L A

出版信息

J Cell Biol. 1985 Feb;100(2):552-7. doi: 10.1083/jcb.100.2.552.

Abstract

Chlorophyll a/b light-harvesting complexes (chl a/b LHC) and photosystem II (PSII) cores were isolated from an octyl glucoside-containing sucrose gradient after solubilization of barley thylakoid membranes with Triton X-100 and octyl glucoside. No cation precipitation step was necessary to collect the chl a/b LHC. PAGE under mildly denaturing and fully denaturing conditions showed that the chl a/b LHC fraction contained chlorophyll-protein complexes CP27, CP29, and CP64. The PSII core material contained CP43 and CP47, and little contamination by other nonpigmented polypeptides. Freeze-fracture electron microscopy of the chl a/b LHC after reconstitution into digalactosyldiglyceride (DG) or phosphatidylcholine (PC) vesicles showed that the protein particles (approximately 7.5 +/- 1.6 nm) were approximately 99 and 90% randomly dispersed, respectively, in the liposomes. Addition of Mg++ produced particle aggregation and membrane adhesion in chl a/b LHC-DG liposomes in a manner analogous to that described for LHC-PC liposomes. Reconstitution of PSII cores into DG vesicles also produced proteoliposomes with randomly dispersed particles (approximately 7.5 +/- 1.6 nm). In contrast, PSII-PC mixtures formed convoluted networks of tubular membranes that exhibited very few fracture faces. Most of the protein particles (approximately 7.0 +/- 1.5 nm) were seen trapped between, rather than embedded in, the membranes. The interaction between the zwitterionic head group of the phosphatidyl choline and the negatively charged PSII core may be responsible for the unusual membrane structures observed.

摘要

在用Triton X - 100和辛基葡糖苷溶解大麦类囊体膜后,从含辛基葡糖苷的蔗糖梯度中分离出叶绿素a/b捕光复合物(chl a/b LHC)和光系统II(PSII)核心。收集chl a/b LHC无需阳离子沉淀步骤。在温和变性和完全变性条件下的聚丙烯酰胺凝胶电泳(PAGE)表明,chl a/b LHC组分包含叶绿素 - 蛋白复合物CP27、CP29和CP64。PSII核心物质包含CP43和CP47,且几乎没有其他非色素多肽的污染。将chl a/b LHC重构到二半乳糖甘油二酯(DG)或磷脂酰胆碱(PC)囊泡后进行的冷冻蚀刻电子显微镜观察表明,蛋白质颗粒(约7.5±1.6 nm)分别约99%和90%随机分散在脂质体中。添加Mg++会使chl a/b LHC - DG脂质体中的颗粒聚集并产生膜黏附,其方式类似于LHC - PC脂质体中所描述的情况。将PSII核心重构到DG囊泡中也产生了具有随机分散颗粒(约7.5±1.6 nm)的蛋白脂质体。相比之下,PSII - PC混合物形成了很少有断裂面的管状膜的复杂网络。大多数蛋白质颗粒(约7.0±1.5 nm)被困在膜之间,而不是嵌入膜中。磷脂酰胆碱的两性离子头部基团与带负电荷的PSII核心之间的相互作用可能是观察到异常膜结构的原因。

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