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多孔介质中蛋白质晶体异质成核的实验与理论

Experiment and theory for heterogeneous nucleation of protein crystals in a porous medium.

作者信息

Chayen Naomi E, Saridakis Emmanuel, Sear Richard P

机构信息

Biological Structure and Function Section, Division of Biomedical Sciences, Sir Alexander Fleming Building, Imperial College London, London SW7 2AZ, United Kingdom.

出版信息

Proc Natl Acad Sci U S A. 2006 Jan 17;103(3):597-601. doi: 10.1073/pnas.0504860102. Epub 2006 Jan 6.

Abstract

The determination of high-resolution structures of proteins requires crystals of suitable quality. Because of the new impetus given to structural biology by structural genomics/proteomics, the problem of crystallizing proteins is becoming increasingly acute. There is therefore an urgent requirement for the development of new efficient methods to aid crystal growth. Nucleation is the crucial step that determines the entire crystallization process. Hence, the holy grail is to design a "universal nucleant," a substrate that induces the nucleation of crystals of any protein. We report a theory for nucleation on disordered porous media and its experimental testing and validation using a mesoporous bioactive gel-glass. This material induced the crystallization of the largest number of proteins ever crystallized using a single nucleant. The combination of the model and the experimental results opens up the scope for the rational design of nucleants, leading to alternative means of controlling crystallization.

摘要

蛋白质高分辨率结构的测定需要具备合适质量的晶体。由于结构基因组学/蛋白质组学为结构生物学带来了新的推动力,蛋白质结晶问题正变得日益严峻。因此,迫切需要开发新的高效方法来辅助晶体生长。成核是决定整个结晶过程的关键步骤。因此,理想的目标是设计一种“通用成核剂”,即一种能诱导任何蛋白质晶体成核的底物。我们报告了一种关于无序多孔介质上成核的理论,并使用介孔生物活性凝胶玻璃对其进行了实验测试和验证。这种材料诱导结晶的蛋白质数量是使用单一成核剂所结晶的蛋白质中最多的。该模型与实验结果相结合,为合理设计成核剂开辟了空间,从而带来了控制结晶的替代方法。

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