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Location of the cyclohexene ring of the chromophore of bacteriorhodopsin by neutron diffraction with selectively deuterated retinal

机译:选择性氘化视网膜的中子衍射对细菌视紫红质发色团环己烯环的定位

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摘要

We report on the location of the cyclohexene ring of the retinylidene chromophore of bacteriorhodopsin projected onto the plane of the membrane. For this purpose, partially deuterated retinal was synthesized containing 11 deuterons at the following positions of the cyclohexene ring: one at C-2, two at C-4, three at C-16, three at C-17, and two at C-18. The partially deuterated retinal was incorporated biosynthetically during growth of the bacteria by using the mutant JW5, which is deficient in the synthesis of retinal. Undeuterated samples were prepared in the same way. Characterization by x-ray diffraction and absorption spectroscopy showed that these samples are identical to native purple membranes as judged by these criteria. A Fourier difference map was calculated from the differences in in-plane diffraction intensities between the deuterated and undeuterated dark-adapted membrane samples. Model calculations showed that the observed difference density had the amplitude expected for a label containing 11 deuterons. At 8.7 Å resolution, the map shows one major peak with the center of mass of the deuterated ring in the interior of the molecule between helices 3, 4, 5, and 6. Based on this result and on our previous work on the location of the middle of the polyene chain, we conclude that the COOH-terminal helix G, to which retinal is attached at lysine-216, is either helix 2 or helix 6.
机译:我们报告了细菌视紫红质的视黄叉生色团的环己烯环的位置投射到膜的平面上。为此目的,合成了部分氘代的视网膜,在环己烯环的以下位置包含11个氘核:一个在C-2,两个在C-4,三个在C-16,三个在C-17和两个在C- 18岁通过使用突变体JW5,部分氘化的视网膜在细菌生长过程中被生物合成并入,该突变体JW5缺乏视网膜的合成能力。以相同方式制备未氘化的样品。通过X射线衍射和吸收光谱表征表明,这些样品与通过这些标准判断的天然紫色膜相同。从氘化和未氘化的暗适应膜样品之间的面内衍射强度差异计算傅立叶差异图。模型计算表明,对于包含11个氘核的标记,观察到的差异密度具有预期的幅度。在8.7Å分辨率下,该图谱显示了一个主峰,氘代环的质心在螺旋3、4、5和6之间的分子内部。根据此结果以及我们先前在位置上的研究在多烯链的中间,我们得出结论,在赖氨酸216上连接视网膜的COOH末端螺旋G是螺旋2或螺旋6。

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