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利用交联作为距离约束,对大型蛋白质组装体进行自动化结构建模。

Automated structure modeling of large protein assemblies using crosslinks as distance restraints.

机构信息

Institut Pasteur, Unité de Bioinformatique Structurale, CNRS UMR 3528, Département de Biologie Structurale et Chimie, Paris, France.

European Molecular Biology Laboratory, Structural and Computational Biology Unit, Heidelberg, Germany.

出版信息

Nat Methods. 2016 Jun;13(6):515-20. doi: 10.1038/nmeth.3838. Epub 2016 Apr 25.

Abstract

Crosslinking mass spectrometry is increasingly used for structural characterization of multisubunit protein complexes. Chemical crosslinking captures conformational heterogeneity, which typically results in conflicting crosslinks that cannot be satisfied in a single model, making detailed modeling a challenging task. Here we introduce an automated modeling method dedicated to large protein assemblies ('XL-MOD' software is available at http://aria.pasteur.fr/supplementary-data/x-links) that (i) uses a form of spatial restraints that realistically reflects the distribution of experimentally observed crosslinked distances; (ii) automatically deals with ambiguous and/or conflicting crosslinks and identifies alternative conformations within a Bayesian framework; and (iii) allows subunit structures to be flexible during conformational sampling. We demonstrate our method by testing it on known structures and available crosslinking data. We also crosslinked and modeled the 17-subunit yeast RNA polymerase III at atomic resolution; the resulting model agrees remarkably well with recently published cryoelectron microscopy structures and provides additional insights into the polymerase structure.

摘要

交联质谱分析越来越多地用于多亚基蛋白质复合物的结构特征分析。化学交联可以捕获构象异质性,这通常会导致无法在单个模型中满足的冲突交联,使得详细建模成为一项具有挑战性的任务。在这里,我们引入了一种专门用于大型蛋白质组装体的自动化建模方法(“XL-MOD”软件可在 http://aria.pasteur.fr/supplementary-data/x-links 获得),该方法 (i) 使用一种空间限制形式,真实地反映了实验观察到的交联距离的分布;(ii) 自动处理模糊和/或冲突的交联,并在贝叶斯框架内识别替代构象;以及 (iii) 允许亚基结构在构象采样过程中具有灵活性。我们通过在已知结构和可用交联数据上测试该方法来证明其有效性。我们还对原子分辨率的 17 亚基酵母 RNA 聚合酶 III 进行了交联和建模;得到的模型与最近发表的冷冻电镜结构非常吻合,并为聚合酶结构提供了更多的见解。

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