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蛋白质电子晶体学中的直接相位测定:水通道蛋白形成通道的整合膜蛋白。

Direct phase determination in protein electron crystallography: aquaporin channel-forming integral membrane protein.

作者信息

Dorset D L, Jap B K

机构信息

Electron Diffraction Department, Hauptman-Woodward Medical Research Institute, 73 High Street, Buffalo, NY 14203, USA.

出版信息

Acta Crystallogr D Biol Crystallogr. 1998 Jul 1;54(Pt 4):615-21. doi: 10.1107/s0907444997018982.

Abstract

The location of helix sites in the projected structure of the aquaporin channel-forming integral membrane protein from bovine red blood cells was determined by multisolution direct methods to a mean accuracy of +/-1.9 A, based on hk0 electron diffraction data extending to 6 A. The structure was assumed to be composed of pseudo-atoms, corresponding to the helix cross sections, and after re-scaling, normalized structure factors were used to order summation operatorn triples according to the A values. Initial phases were found by symbolic addition with algebraic unknowns. Probable solutions could be isolated by an overall Luzzati test for density flatness and restrictions on local density extremes. The best solution was identified by matching Patterson functions, generated from the trial map density sites, to the one calculated from observed intensities.

摘要

基于延伸至6埃的hk0电子衍射数据,采用多解直接法确定了来自牛红细胞的水通道蛋白形成通道的整合膜蛋白投影结构中螺旋位点的位置,平均精度为±1.9埃。该结构被假定为由对应于螺旋横截面的伪原子组成,重新缩放后,使用归一化结构因子根据A值对求和算子三元组进行排序。通过带有代数未知数的符号相加找到初始相位。可以通过对密度平整度的整体卢扎蒂检验和对局部密度极值的限制来分离可能的解。通过将从试验图密度位点生成的帕特森函数与根据观察到的强度计算出的函数进行匹配,确定最佳解。

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