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线粒体通道电压依赖性阴离子通道(VDAC)晶体阵列的表面形貌和分子化学计量

Surface topography and molecular stoichiometry of the mitochondrial channel, VDAC, in crystalline arrays.

作者信息

Thomas L, Kocsis E, Colombini M, Erbe E, Trus B L, Steven A C

机构信息

Department of Zoology, University of Maryland, College Park 20742.

出版信息

J Struct Biol. 1991 Apr;106(2):161-71. doi: 10.1016/1047-8477(91)90085-b.

Abstract

The mitochondrial outer membrane contains a protein, called VDAC, that forms large aqueous pores. In Neurospora crassa outer membranes, VDAC forms two-dimensional crystalline arrays whose size and frequency can be greatly augmented by lipase treatment of these membranes (C. Mannella, Science 224, 165, 1984). Fourier filtration and surface reconstruction of freeze-dried/shadowed (45 degrees) arrays produced detailed images of two populations of crystals, whose lattices are mirror images of each other. Most likely, this technique has revealed both surfaces of the same two-dimensional crystal with lattice parameters: a = 12.3 +/- 0.1 nm, b = 11.2 +/- 0.1 nm, and theta = 109 +/- 1 degree. Three-dimensional reconstructions of the surface reliefs on both sides of the crystal show them to be very similar. The majority of the protein forming the channel appears to be at or below the level of the membrane. To address the issue of the number of 30-kDa polypeptides that form a VDAC channel, measurements of mass per unit area were carried out by analyzing scanning transmission electron micrographs of unstained, freeze-dried arrays. The crystal form used for mass analysis contained the same motif of six stain-accumulating centers per unit cell, with p2 symmetry as in the oblique configuration, but it had a different orientation relative to the lattice lines. These data yielded a surface density of 1.9 +/- 0.2 kDa/nm2, indicating that there is a one-to-one ratio between VDAC polypeptides and the channels visualized in filtered electron micrographs, and that VDAC membrane crystals contain 68% protein and 32% lipid by mass.

摘要

线粒体外膜含有一种名为电压依赖性阴离子通道(VDAC)的蛋白质,它能形成大的水性孔道。在粗糙脉孢菌的外膜中,VDAC形成二维晶体阵列,通过对这些膜进行脂肪酶处理,其大小和频率可大幅增加(C. 曼内拉,《科学》224, 165, 1984)。对冻干/投影(45度)阵列进行傅里叶滤波和表面重建,得到了两种晶体群体的详细图像,它们的晶格互为镜像。很可能,这项技术揭示了同一二维晶体的两个表面,其晶格参数为:a = 12.3 +/- 0.1纳米,b = 11.2 +/- 0.1纳米,θ = 109 +/- 1度。对晶体两侧表面浮雕的三维重建显示它们非常相似。形成通道的大部分蛋白质似乎位于膜的水平或以下。为了解决形成VDAC通道的30 kDa多肽数量问题,通过分析未染色、冻干阵列的扫描透射电子显微照片进行了单位面积质量测量。用于质量分析的晶体形式每个晶胞包含相同的六个染色积累中心基序,具有与倾斜构型相同的p2对称性,但相对于晶格线有不同的取向。这些数据得出表面密度为1.9 +/- 0.2 kDa/nm2,表明VDAC多肽与在滤波电子显微照片中可视化的通道之间存在一对一的比例,并且VDAC膜晶体按质量计含有68%的蛋白质和32%的脂质。

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