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一种用于蛋白质封装的简单标记系统。

A simple tagging system for protein encapsulation.

作者信息

Seebeck Florian P, Woycechowsky Kenneth J, Zhuang Wei, Rabe Jürgen P, Hilvert Donald

机构信息

Laboratorium für Organische Chemie, ETH Zürich, Hönggerberg HCI F337, CH-8093, Zürich, Switzerland.

出版信息

J Am Chem Soc. 2006 Apr 12;128(14):4516-7. doi: 10.1021/ja058363s.

Abstract

Molecular containers that encapsulate specific cargo can be useful for many natural and non-natural processes. We report a simple system, based on charge complementarity, for the encapsulation of appropriately tagged proteins within an engineered, proteinaceous capsid. Four negative charges per monomer were added to the lumazine synthase from Aquifex aeolicus (AaLS). The capsids formed by the engineered AaLS associate with green fluorescent protein bearing a positively charged deca-arginine tag upon coproduction in Escherichia coli. Analytical ultracentrifugation and scanning force microscopy studies indicated that the engineered AaLS retains the ability to form capsids, but that their average size was substantially increased. The success of this strategy demonstrates that both the container and guest components of protein-based encapsulation systems can be convergently designed in a straightforward manner, which may help to extend their versatility.

摘要

能够包裹特定货物的分子容器可用于许多自然和非自然过程。我们报告了一个基于电荷互补性的简单系统,用于在工程化的蛋白质衣壳内包裹带有适当标签的蛋白质。从嗜热栖热菌(AaLS)中提取的鲁比嗪合酶每个单体添加了四个负电荷。在大肠杆菌中共表达时,由工程化AaLS形成的衣壳与带有带正电荷的十聚精氨酸标签的绿色荧光蛋白结合。分析超速离心和扫描力显微镜研究表明,工程化AaLS保留了形成衣壳的能力,但其平均尺寸大幅增加。该策略的成功表明,基于蛋白质的封装系统的容器和客体组件都可以以直接的方式进行汇聚设计,这可能有助于扩展其通用性。

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