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用于测定大分子旋转对称性的改进方法。

Improved methods for determination of rotational symmetries in macromolecules.

作者信息

Kocsis E, Cerritelli M E, Trus B L, Cheng N, Steven A C

机构信息

Laboratory of Structural Biology, NIAMS, National Institutes of Health, Bethesda, MD 20892-2755, USA.

出版信息

Ultramicroscopy. 1995 Sep;60(2):219-28. doi: 10.1016/0304-3991(95)00070-2.

Abstract

Rotational symmetries of macromolecules are most clearly perceived in the en face projection and may be assessed by inspection of rotational power spectra calculated from electron micrographs of individual particles. However, if the symmetry is not contrasted strongly, this procedure may be inconclusive since the relevant peak may not be convincingly higher than other spectral components. To some extent, this is a sampling problem since the number of repeating elements involved is usually small. We have devised more sensitive statistical tests for rotational symmetry that pool the information contents of entire populations of particles. Both tests involve combining the rotational spectra of many particles and comparing them with the spectra of surrounding background areas. One method is based on the well known t-test which estimates whether two populations differ at a given significance level. In the second test, the ratio between the intensity of each component of the rotational spectrum and the average corresponding intensity for background areas is calculated, and thence, the cumulative product of these ratios over all particles in the data set. If a symmetry is present, this product gradually diverges; otherwise, it converges to zero. As a practical trial, the tests were applied to micrographs of negatively stained hexons of herpes simplex virus and confirmed their 6-fold symmetry. Applied to negatively stained "connector" proteins of bacteriophage T7 purified from a plasmid expression system, both algorithms detected polymorphism with distinct subpopulations of both 13-fold and 12-fold connectors.

摘要

大分子的旋转对称性在正视图投影中最为明显,可通过检查从单个颗粒的电子显微照片计算出的旋转功率谱来评估。然而,如果对称性对比不强烈,这个过程可能没有定论,因为相关峰可能并不比其他光谱成分高得令人信服。在某种程度上,这是一个抽样问题,因为所涉及的重复元素数量通常很少。我们设计了更灵敏的旋转对称性统计测试,将整个颗粒群体的信息内容汇总起来。这两种测试都涉及合并许多颗粒的旋转光谱,并将它们与周围背景区域的光谱进行比较。一种方法基于著名的t检验,该检验估计两个群体在给定显著性水平上是否存在差异。在第二种测试中,计算旋转光谱各成分的强度与背景区域平均相应强度之间的比率,然后计算数据集中所有颗粒这些比率的累积乘积。如果存在对称性,这个乘积会逐渐发散;否则,它会收敛到零。作为实际试验,这些测试应用于单纯疱疹病毒负染六邻体的显微照片,并证实了它们的六重对称性。应用于从质粒表达系统纯化的噬菌体T7的负染“连接蛋白”,两种算法都检测到了具有13倍和12倍连接蛋白不同亚群的多态性。

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