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首页> 外文期刊>Journal of Electron Microscopy >3D imaging and quantitative analysis of small solubilized membrane proteins and their complexes by transmission electron microscopy.
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3D imaging and quantitative analysis of small solubilized membrane proteins and their complexes by transmission electron microscopy.

机译:通过透射电子显微镜对小分子可溶性膜蛋白及其复合物进行3D成像和定量分析。

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摘要

Inherently unstable, detergent-solubilized membrane protein complexes can often not be crystallized. For complexes that have a mass of >300 kDa, cryo-electron microscopy (EM) allows their three-dimensional (3D) structure to be assessed to a resolution that makes secondary structure elements visible in the best case. However, many interesting complexes exist whose mass is below 300 kDa and thus need alternative approaches. Two methods are reviewed: (i) Mass measurement in a scanning transmission electron microscope, which has provided important information on the stoichiometry of membrane protein complexes. This technique is applicable to particulate, filamentous and sheet-like structures. (ii) 3D-EM of negatively stained samples, which determines the molecular envelope of small membrane protein complexes. Staining and dehydration artifacts may corrupt the quality of the 3D map. Staining conditions thus need to be optimized. 3D maps of plant aquaporin SoPIP2;1 tetramers solubilized in different detergents illustrate that the flattening artifact can be partially prevented and that the detergent itself contributes significantly. Another example discussed is the complex of G protein-coupled receptor rhodopsin with its cognate G protein transducin.
机译:内在不稳定的,去污剂溶解的膜蛋白复合物通常不能结晶。对于质量> 300 kDa的复合物,低温电子显微镜(EM)允许将其三维(3D)结构评估为可以使二级结构元素在最佳情况下可见的分辨率。但是,存在许多质量低于300 kDa的有趣复合物,因此需要其他方法。审查了两种方法:(i)在扫描透射电子显微镜中进行质量测量,它提供了有关膜蛋白复合物化学计量的重要信息。该技术适用于颗粒状,丝状和片状结构。 (ii)负染色样品的3D-EM,它决定了小膜蛋白复合物的分子包膜。染色和脱水伪影可能会破坏3D地图的质量。因此需要优化染色条件。在不同去污剂中溶解的植物水通道蛋白SoPIP2; 1四聚体的3D图谱表明,可以部分防止变平伪影,并且去污剂本身也起了很大作用。讨论的另一个例子是G蛋白偶联受体视紫红质与其同源G蛋白转导蛋白的复合物。

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