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De novo design of a fluorescence - activating β-barrel

机译:从头开始设计荧光激活的β-桶

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The regular arrangements of beta-strands around a central axis in beta-barrels and of a-helices in coiled coils contrast with the irregular tertiary structures of most globular proteins, and have fascinated structural biologists since they were first discovered. Simple parametric models have been used to design a wide range of a-helical coiled-coil structures, but to date there has been no success with beta-barrels. Here we show that accurate de novo design of beta-barrels requires considerable symmetry-breaking to achieve continuous hydrogen-bond connectivity and eliminate backbone strain. We then build ensembles of beta-barrel backbone models with cavity shapes that match the fluorogenic compound DFHBI, and use a hierarchical grid-based search method to simultaneously optimize the rigid-body placement of DFHBI in these cavities and the identities of the surrounding amino acids to achieve high shape and chemical complementarity. The designs have high structural accuracy and bind and fluorescently activate DFHBI in vitro and in Escherichia coli, yeast and mammalian cells. This de novo design of small-molecule binding activity, using backbones custom-built to bind the ligand, should enable the design of increasingly sophisticated ligand-binding proteins, sensors and catalysts that are not limited by the backbone geometries available in known protein structures.
机译:β-桶中围绕中心轴的β-链的规则排列以及螺旋形线圈中的α-螺旋的排列与大多数球状蛋白质的不规则三级结构形成对比,并且自从首次发现以来就吸引了结构生物学家。简单的参数模型已被用于设计各种各样的a螺旋线圈结构,但是迄今为止,β桶还没有成功。在这里,我们证明了精确的从头开始设计β桶需要打破对称性才能实现连续的氢键连接并消除骨架应力。然后,我们构建具有与荧光化合物DFHBI相匹配的空腔形状的β-桶骨架模型的合奏,并使用基于层次网格的搜索方法来同时优化DFHBI在这些空腔中的刚体位置以及周围氨基酸的身份实现高形状和化学互补性。这些设计具有很高的结构精度,并且可以在体外以及在大肠杆菌,酵母和哺乳动物细胞中结合并荧光激活DFHBI。这种使用小分子结合活性定制的从头设计的小分子结合活性,应能够设计出越来越复杂的配体结合蛋白,传感器和催化剂,而不受已知蛋白结构中可用的骨架几何形状的限制。

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