Direct Observation of Protein Microcrystals in Crystallization Buffer by Atmospheric Scanning Electron Microscopy

被引:15
|
作者
Maruyama, Yuusuke [1 ]
Ebihara, Tatsuhiko [1 ]
Nishiyama, Hidetoshi [2 ]
Konyuba, Yuji [2 ]
Senda, Miki [3 ]
Numaga-Tomita, Takuro [4 ]
Senda, Toshiya [5 ]
Suga, Mitsuo [2 ]
Sato, Chikara [1 ]
机构
[1] Natl Inst Adv Ind Sci & Technol, Biomed Res Inst, Tsukuba, Ibaraki 3058566, Japan
[2] JEOL Ltd, Adv Technol Div, Akishima, Tokyo 1968558, Japan
[3] Japan Biol Informat Consortium JBIC, Struct Guided Drug Dev Project, JBIC Res Inst, Koto Ku, Tokyo 1350064, Japan
[4] NIEHS, NIH, US Dept HHS, Res Triangle Pk, NC 27709 USA
[5] Natl Inst Adv Ind Sci & Technol, Biomedicinal Informat Res Ctr, Koto Ku, Tokyo 1350064, Japan
基金
日本科学技术振兴机构;
关键词
X-ray crystallography; protein crystal; nano-crystal; crystallization screening; environmental cell; TAF-I beta; micro-focus X-ray beams; X-ray free-electron laser; ASEM; ClairScope; ATOMIC-FORCE MICROSCOPY; CRYSTAL-GROWTH; CHANNEL; TISSUES; CELLS;
D O I
10.3390/ijms130810553
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
X-ray crystallography requires high quality crystals above a given size. This requirement not only limits the proteins to be analyzed, but also reduces the speed of the structure determination. Indeed, the tertiary structures of many physiologically important proteins remain elusive because of the so-called "crystallization bottleneck". Once microcrystals have been obtained, crystallization conditions can be optimized to produce bigger and better crystals. However, the identification of microcrystals can be difficult due to the resolution limit of optical microscopy. Electron microscopy has sometimes been utilized instead, with the disadvantage that the microcrystals usually must be observed in vacuum, which precludes the usage for crystal screening. The atmospheric scanning electron microscope (ASEM) allows samples to be observed in solution. Here, we report the use of this instrument in combination with a special thin-membrane dish with a crystallization well. It was possible to observe protein crystals of lysozyme, lipase B and a histone chaperone TAF-I beta in crystallization buffers, without the use of staining procedures. The smallest crystals observed with ASEM were a few mu m in width, and ASEM can be used with non-transparent solutions. Furthermore, the growth of salt crystals could be monitored in the ASEM, and the difference in contrast between salt and protein crystals made it easy to distinguish between these two types of microcrystals. These results indicate that the ASEM could be an important new tool for the screening of protein microcrystals.
引用
收藏
页码:10553 / 10567
页数:15
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