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光系统II的捕光叶绿素蛋白复合体。其在光合膜中的位置。

The light-harvesting chlorpohyll-protein complex of photosystem II. Its location in the photosynthetic membrane.

作者信息

Miller K R, Miller G J, McIntyre K R

出版信息

J Cell Biol. 1976 Nov;71(2):624-38. doi: 10.1083/jcb.71.2.624.

Abstract

We have investigated the structure of the photosynthetic membrane in a mutant of barley known to lack a chlorophyll-binding protein. This protein is thought to channel excitation energy to photosystem II, and is known as the "light-harvesting chlorophyll-protein complex." Extensive stacking of thylakoids into grana occurs in both mutant and wild-type chloroplasts. Examination of membrane internal structure by freeze-fracturing indicates that only slight differences exist between the fracture faces of mutant and wild-type membranes. These differences are slight reductions in the size of particles visible on the EFs fracture face, and in the number of particles seen on the PFs fracture face. No differences can be detected between mutant and wild-type on the etched out surface of the membrane. In contrast, tetrameric particles visible on the etched inner surface of wild-type thylakoids are extremely difficult to recognize on similar surfaces of the mutant. These particles can be recognized on inner surfaces of the mutant membranes when they are organized into regular lattices, but these lattices show a much closer particle-to-particle spacing than similar lattices in wild-type membranes. Although several interpretations of these data are possible, these observations are consistent with the proposal that the light-harvesting chlorophyll-protein complex of photosystem II is bound to the tetramer (which is visible on the EFs face as a single particle) near the inner surface of the membrane. The large tetramer, which other studies have shown to span the thylakoid membrane, may represent an assembly of protein, lipid, and pigment comprising all the elements of the photosystem II reaction. A scheme is presented which illustrates one possibility for the light reaction across the photosynthetic membrane.

摘要

我们研究了大麦一个突变体的光合膜结构,已知该突变体缺乏一种叶绿素结合蛋白。这种蛋白被认为能将激发能传递到光系统II,被称为“捕光叶绿素蛋白复合体”。突变体和野生型叶绿体中都存在类囊体大量堆叠形成基粒的现象。通过冷冻断裂对膜内部结构进行检查表明,突变体膜和野生型膜的断裂面之间仅存在细微差异。这些差异表现为在EFs断裂面上可见颗粒大小略有减小,以及在PFs断裂面上可见颗粒数量略有减少。在膜的蚀刻表面上,突变体和野生型之间未检测到差异。相比之下,在野生型类囊体蚀刻内表面可见的四聚体颗粒在突变体的类似表面上极难识别。当这些颗粒在突变体膜的内表面组织成规则晶格时可以识别,但这些晶格中颗粒间的间距比野生型膜中类似晶格的间距小得多。尽管对这些数据有几种可能的解释,但这些观察结果与以下提议一致:光系统II的捕光叶绿素蛋白复合体与膜内表面附近的四聚体(在EFs面上可见为单个颗粒)结合。其他研究表明,大的四聚体跨越类囊体膜,可能代表了由光系统II反应的所有元素组成的蛋白质、脂质和色素的组装体。本文提出了一个示意图,说明了光合膜上光反应的一种可能性。

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本文引用的文献

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Quantasome: Size and Composition.Quanta 体:大小与组成。
Science. 1964 May 22;144(3621):1009-11. doi: 10.1126/science.144.3621.1009.
4
CHLOROPHYLL STUDIES ON BARLEY MUTANTS.大麦突变体的叶绿素研究
Plant Physiol. 1950 Apr;25(2):294-306. doi: 10.1104/pp.25.2.294.

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