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Homogeneous batch micro-crystallization of proteins from ammonium sulfate

机译:齐次批micro-crystallization的蛋白质从硫酸铵

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The emergence of X-ray free-electron lasers has led to the development of serial macromolecular crystallography techniques, making it possible to study smaller and more challenging crystal systems and to perform time-resolved studies on fast time scales. For most of these studies the desired crystal size is limited to a few micrometres, and the generation of large amounts of nanocrystals or microcrystals of defined size has become a bottleneck for the wider implementation of these techniques. Despite this, methods to reliably generate microcrystals and fine-tune their size have been poorly explored. Working with three different enzymes, L-aspartate α-decarboxylase, copper nitrite reductase and copper amine oxidase, the precipitating properties of ammonium sulfate were exploited to quickly transition from known vapour-diffusion conditions to reproducible, large-scale batch crystallization, circumventing the tedious determination of phase diagrams. Furthermore, the specific ammonium sulfate concentration was used to fine-tune the crystal size and size distribution. Ammonium sulfate is a common precipitant in protein crystallography, making these findings applicable to many crystallization systems to facilitate the production of large amounts of microcrystals for serial macromolecular crystallography experiments.
机译:x射线自由电子激光的出现导致连环高分子的发展晶体学技术,使成为可能研究更小,更具挑战性的晶体系统和执行时间分辨的研究快时间尺度。理想晶体大小是有限的微米,大量的一代纳米晶体或微晶核尺寸定义已经成为更广泛的瓶颈这些技术的实现。可靠地生成微晶核和方法探索调整它们的大小一直不佳。使用三种不同的酶,L-aspartateα脱羧酶、铜亚硝酸还原酶和铜胺氧化酶、沉淀硫酸铵被剥削的属性从已知vapour-diffusion迅速转变可再生的条件,大规模的批处理结晶,绕过乏味测定相图。使用特定的硫酸铵浓度来调整晶体尺寸和大小分布。在蛋白质结晶学沉淀剂,使这些发现适用于许多结晶系统以促进大型的生产大量的微晶核系列大分子晶体学实验。

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