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本文引用的文献

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Circular dichroic spectrum of the L form and the blue light product of the m form of purple membrane.L 型紫膜和 M 型紫膜蓝光产物的圆二色性光谱。
Biophys J. 1987 Jan;51(1):145-8. doi: 10.1016/S0006-3495(87)83319-2.
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Large Scale Global Structural Changes of the Purple Membrane during the Photocycle.在光循环过程中紫色膜的大规模全球结构变化。
Biophys J. 1985 Apr;47(4):497-507. doi: 10.1016/S0006-3495(85)83943-6.
3
High-sensitivity neutron diffraction of membranes: Location of the Schiff base end of the chromophore of bacteriorhodopsin.高灵敏度中子衍射膜:细菌视紫红质发色团的席夫碱末端的位置。
Proc Natl Acad Sci U S A. 1988 Apr;85(7):2146-50. doi: 10.1073/pnas.85.7.2146.
4
Location of the cyclohexene ring of the chromophore of bacteriorhodopsin by neutron diffraction with selectively deuterated retinal.用选择性氘化视黄醛的中子衍射确定菌紫质发色团中环己烯环的位置。
Proc Natl Acad Sci U S A. 1986 Oct;83(20):7746-50. doi: 10.1073/pnas.83.20.7746.
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Electron diffraction analysis of structural changes in the photocycle of bacteriorhodopsin.细菌视紫红质光循环中结构变化的电子衍射分析
EMBO J. 1993 Jan;12(1):1-8. doi: 10.1002/j.1460-2075.1993.tb05625.x.
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Distorted structure of the retinal chromophore in bacteriorhodopsin resolved by 2H-NMR.通过2H-NMR解析细菌视紫红质中视网膜发色团的扭曲结构。
Biochemistry. 1994 May 10;33(18):5370-5. doi: 10.1021/bi00184a003.
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Time-resolved x-ray diffraction study of photostimulated purple membrane.光刺激紫色膜的时间分辨X射线衍射研究
Biophys J. 1985 Mar;47(3):387-93. doi: 10.1016/S0006-3495(85)83930-8.
8
A neutron diffraction study on the location of the polyene chain of retinal in bacteriorhodopsin.关于细菌视紫红质中视黄醛多烯链位置的中子衍射研究。
Proc Natl Acad Sci U S A. 1985 May;82(10):3227-31. doi: 10.1073/pnas.82.10.3227.
9
Orientation of the bacteriorhodopsin chromophore probed by polarized Fourier transform infrared difference spectroscopy.通过偏振傅里叶变换红外差光谱法探测细菌视紫红质发色团的取向
Biochemistry. 1986 Dec 2;25(24):7793-8. doi: 10.1021/bi00372a002.
10
Electron diffraction analysis of the M412 intermediate of bacteriorhodopsin.细菌视紫红质M412中间体的电子衍射分析。
Biophys J. 1986 Nov;50(5):913-20. doi: 10.1016/S0006-3495(86)83532-9.

光诱导异构化导致细菌视紫红质M中间体中发色团倾斜增加:一项中子衍射研究。

Light-induced isomerization causes an increase in the chromophore tilt in the M intermediate of bacteriorhodopsin: a neutron diffraction study.

作者信息

Hauss T, Büldt G, Heyn M P, Dencher N A

机构信息

Department of Physics, Freie Universität Berlin, Germany.

出版信息

Proc Natl Acad Sci U S A. 1994 Dec 6;91(25):11854-8. doi: 10.1073/pnas.91.25.11854.

DOI:10.1073/pnas.91.25.11854
PMID:7991546
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC45334/
Abstract

Bacteriorhodopsin (BR) was regenerated with two selectively deuterated retinals, one with 11 deuterons in the beta-ionone ring (D11) and the other with 5 deuterons (D5) at the end of the polyene chain closest to the Schiff base at carbon atoms C-14, C-15, and C-20. Both label positions (centers of deuteration) were obtained from difference Fourier maps of projections onto the plane of the membrane by neutron diffraction at 90 K, both in the light-adapted ground-state BR568 and in the photocycle intermediate M412. To retard the decay of M412, purple membrane films were soaked in 0.1 M or 1 M guanidine hydrochloride at pH 9.6. M412 was produced by illuminating oriented membrane films at physiological temperature (278 K), followed by rapid cooling to 90 K in the absence of light. The results show that in the projected structure the ring position is unaltered during the transition from BR568 to M412, whereas the position of the D5 label shifts by 1.4 +/- 0.9 A toward the ring. The shortened interlabel distance in the projected structure for the M412 state implies that as a result of the all-trans/13-cis isomerization, the C-5 to C-13 part of the polyene chain tilts out of the plane of the membrane toward the cytoplasm by about 11 degrees +/- 6 degrees. Pairwise comparison of data sets with the same retinal for the two photocycle states M412 and BR568 leads to four difference-density maps for the protein, which are in agreement with previous work. They show changes in the protein density near helices G and F.

摘要

用两种选择性氘代视黄醛再生细菌视紫红质(BR),一种在β-紫罗兰酮环中有11个氘原子(D11),另一种在多烯链最靠近席夫碱的末端碳原子C-14、C-15和C-20处有5个氘原子(D5)。这两个标记位置(氘代中心)是通过在90K下用中子衍射对膜平面投影的差分傅里叶图获得的,无论是在光适应的基态BR568还是在光循环中间体M412中。为了延缓M412的衰变,将紫膜膜片浸泡在pH 9.6的0.1M或1M盐酸胍中。通过在生理温度(278K)下照射取向的膜片,然后在无光条件下快速冷却至90K来产生M412。结果表明,在投影结构中,从BR568转变为M412期间,环位置不变,而D5标记的位置向环移动了1.4±0.9 Å。M412状态投影结构中缩短的标记间距离意味着,由于全反式/13-顺式异构化,多烯链的C-5至C-13部分向细胞质倾斜出膜平面约11°±6°。对光循环状态M412和BR568的相同视黄醛数据集进行成对比较,得到了蛋白质的四张差分密度图,与先前的工作一致。它们显示了螺旋G和F附近蛋白质密度的变化。