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[带负电荷蛋白质笼的结构与自组装]

[Structure and Self-assembly of Negatively Supercharged Protein Cages].

作者信息

Sasaki Eita, Hilvert Donald

机构信息

Graduate School of Agricultural and Life Sciences, The University of Tokyo.

Department of Chemistry and Applied Biosciences, Laboratory of Organic Chemistry, ETH Zurich.

出版信息

Yakugaku Zasshi. 2019;139(2):199-208. doi: 10.1248/yakushi.18-00169-2.

DOI:10.1248/yakushi.18-00169-2
PMID:30713229
Abstract

Proteins are excellent materials for constructing nano- to micro-meter sized compartments. For example, in nature, hollow spherical shells made of proteins, called protein cages, are widespread. Prominent examples include viruses, ferritins, carboxysomes, and others. Protein cages designed and engineered in the laboratory have also gained recent attention because of their potential use in synthetic biology, materials science, and medicine. Here, we show that engineered variants of lumazine synthase (LS) from Aquifex aeolicus self-assemble into porous shell-like structures, with striking size-expansion from the original dodecahedron composed of 12 pentamer subunits. Cryo-electron microscopy (EM) analysis has revealed that pentamers are the basic assembly units, although small conformational changes in each subunit lead to final expanded architectures composed of 36 and 72 pentamers. The underlying conformational changes likely arise from electrostatic repulsion between anionic residues originally introduced at the lumenal surface of the LS cage to encapsulate positively charged guest molecules. The plastic nature of the LS cage structure was also explored using a positively supercharged variant of the green fluorescent protein GFP(+36) as an assembly mediator. By controlling the favorable electrostatic interactions between the negatively charged LS cage and the positively charged mediator, multishell structures were created, as previously observed in some virus-like particles. These results highlight the potential of engineered LS cages for various future applications, including drug delivery and bioimaging.

摘要

蛋白质是构建纳米到微米级隔室的优质材料。例如,在自然界中,由蛋白质构成的空心球形外壳,即所谓的蛋白质笼,广泛存在。突出的例子包括病毒、铁蛋白、羧基体等。实验室设计和改造的蛋白质笼由于其在合成生物学、材料科学和医学中的潜在用途,近来也受到了关注。在此,我们展示了来自嗜热栖热菌的鲁比嗪合酶(LS)的工程变体自组装成多孔的壳状结构,与由12个五聚体亚基组成的原始十二面体相比,尺寸显著扩大。冷冻电子显微镜(EM)分析表明,五聚体是基本的组装单元,尽管每个亚基的微小构象变化导致最终由36个和72个五聚体组成的扩展结构。潜在的构象变化可能源于最初在LS笼腔表面引入的阴离子残基之间的静电排斥,以封装带正电荷的客体分子。还使用绿色荧光蛋白GFP(+36)的带正电的变体作为组装介质,探索了LS笼结构的可塑性。通过控制带负电的LS笼与带正电的介质之间有利的静电相互作用,创造出了多壳结构,正如之前在一些病毒样颗粒中观察到的那样。这些结果突出了工程化LS笼在包括药物递送和生物成像在内的各种未来应用中的潜力。

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