Feasibility of imaging living cells at subnanometer resolutions by ultrafast X-ray diffraction

被引:75
作者
Bergh, Magnus [1 ]
Huldt, Gosta [1 ]
Timneanu, Nicusor [1 ]
Maia, Filipe R. N. C. [1 ]
Hajdu, Janos [1 ,2 ]
机构
[1] Uppsala Univ, Inst Cell & Mol Biol, Lab Mol Biophys, S-75124 Uppsala, Sweden
[2] Stanford Linear Accelerator Ctr, Menlo Pk, CA USA
基金
瑞典研究理事会;
关键词
D O I
10.1017/S003358350800471X
中图分类号
Q6 [生物物理学];
学科分类号
071011 ;
摘要
Detailed structural investigations on living cells are problematic because existing structural methods cannot reach high resolutions on non-reproducible objects. Illumination with an ultrashort and extremely bright X-ray pulse can outrun key damage processes over a very short period. This can be exploited to extend the diffraction signal to the highest possible resolution in flash diffraction experiments. Here we present an analysis or the interaction of a very intense and very short X-ray pulse with a living cell, using a non-equilibrium population kinetics plasma code with radiation transfer. Each element in the evolving plasma is modeled by numerous states to monitor changes in the atomic populations as a function of pulse length, wavelength, and fluence. The model treats photoionization, impact ionization, Auger decay, recombination, and inverse bremsstrahlung by solving rate equations in a self-consistent manner and describes hydrodynamic expansion through the ion sound speed, The results show that subnanometer resolutions could be reached on micron-sized cells in a diffraction-limited geometry at wavelengths between 0.75 and 1.5 nm and at fluences of 10(11)-10(12) photonS mu M (2) in less than 10 fs. Subnanometer resolutions could also be achieved with harder X-rays at higher fluences. We discuss experimental and computational strategies to obtain depth information about the object in flash diffraction experiments.
引用
收藏
页码:181 / 204
页数:24
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