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串行X射线晶体学中的剂量、曝光时间和分辨率。

Dose, exposure time and resolution in serial X-ray crystallography.

作者信息

Starodub D, Rez P, Hembree G, Howells M, Shapiro D, Chapman H N, Fromme P, Schmidt K, Weierstall U, Doak R B, Spence J C H

机构信息

Department of Physics, Arizona State University, PO Box 871504, Tempe, AZ 85287-1504, USA.

出版信息

J Synchrotron Radiat. 2008 Jan;15(Pt 1):62-73. doi: 10.1107/S0909049507048893. Epub 2007 Dec 18.

DOI:10.1107/S0909049507048893
PMID:18097080
Abstract

The resolution of X-ray diffraction microscopy is limited by the maximum dose that can be delivered prior to sample damage. In the proposed serial crystallography method, the damage problem is addressed by distributing the total dose over many identical hydrated macromolecules running continuously in a single-file train across a continuous X-ray beam, and resolution is then limited only by the available molecular and X-ray fluxes and molecular alignment. Orientation of the diffracting molecules is achieved by laser alignment. The incident X-ray fluence (energy/area) is evaluated that is required to obtain a given resolution from (i) an analytical model, giving the count rate at the maximum scattering angle for a model protein, (ii) explicit simulation of diffraction patterns for a GroEL-GroES protein complex, and (iii) the spatial frequency cut-off of the transfer function following iterative solution of the phase problem, and reconstruction of an electron density map in the projection approximation. These calculations include counting shot noise and multiple starts of the phasing algorithm. The results indicate counting time and the number of proteins needed within the beam at any instant for a given resolution and X-ray flux. An inverse fourth-power dependence of exposure time on resolution is confirmed, with important implications for all coherent X-ray imaging. It is found that multiple single-file protein beams will be needed for sub-nanometer resolution on current third-generation synchrotrons, but not on fourth-generation designs, where reconstruction of secondary protein structure at a resolution of 7 A should be possible with relatively short exposures.

摘要

X射线衍射显微镜的分辨率受限于在样品受损之前所能施加的最大剂量。在提出的串行晶体学方法中,通过将总剂量分布在许多相同的水合大分子上解决了损伤问题,这些大分子以单列形式连续穿过连续的X射线束,然后分辨率仅受可用的分子通量、X射线通量和分子排列的限制。通过激光排列实现衍射分子的取向。通过以下方式评估获得给定分辨率所需的入射X射线注量(能量/面积):(i)一个分析模型,给出模型蛋白质在最大散射角处的计数率;(ii)对GroEL-GroES蛋白质复合物的衍射图案进行显式模拟;(iii)在相位问题的迭代求解以及投影近似下电子密度图的重建之后,传递函数的空间频率截止。这些计算包括计数散粒噪声和相位算法的多次启动。结果表明了对于给定分辨率和X射线通量,计数时间以及在任何时刻束内所需蛋白质的数量。证实了曝光时间与分辨率呈四次方反比关系,这对所有相干X射线成像都具有重要意义。研究发现,对于当前的第三代同步加速器,要实现亚纳米分辨率需要多个单列蛋白质束,但对于第四代设计则不需要,在第四代设计中,以7埃的分辨率重建二级蛋白质结构在相对较短的曝光时间内应该是可行的。

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