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本文引用的文献

1
Structural photoactivation of a full-length bacterial phytochrome.结构光激活全细菌光敏色素。
Sci Adv. 2016 Aug 12;2(8):e1600920. doi: 10.1126/sciadv.1600920. eCollection 2016 Aug.
2
The Crystal Structures of the N-terminal Photosensory Core Module of Agrobacterium Phytochrome Agp1 as Parallel and Anti-parallel Dimers.农杆菌光敏色素Agp1的N端光感受核心模块作为平行和反平行二聚体的晶体结构
J Biol Chem. 2016 Sep 23;291(39):20674-91. doi: 10.1074/jbc.M116.739136. Epub 2016 Jul 26.
3
Crystal Structure of Deinococcus Phytochrome in the Photoactivated State Reveals a Cascade of Structural Rearrangements during Photoconversion.光激活状态下嗜放射栖热菌光敏色素的晶体结构揭示了光转化过程中的一系列结构重排。
Structure. 2016 Mar 1;24(3):448-57. doi: 10.1016/j.str.2016.01.001. Epub 2016 Feb 4.
4
Crystallographic and electron microscopic analyses of a bacterial phytochrome reveal local and global rearrangements during photoconversion.对一种细菌光敏色素的晶体学和电子显微镜分析揭示了光转换过程中的局部和整体重排。
J Biol Chem. 2014 Aug 29;289(35):24573-87. doi: 10.1074/jbc.M114.571661. Epub 2014 Jul 8.
5
Signal amplification and transduction in phytochrome photosensors.光敏色素光传感器中的信号放大和转导。
Nature. 2014 May 8;509(7499):245-248. doi: 10.1038/nature13310. Epub 2014 Apr 30.
6
Ultrafast red light activation of Synechocystis phytochrome Cph1 triggers major structural change to form the Pfr signalling-competent state.超快红光激活集胞藻藻红蛋白 Cph1 引发主要结构变化,形成 Pfr 信号有活性状态。
PLoS One. 2012;7(12):e52418. doi: 10.1371/journal.pone.0052418. Epub 2012 Dec 26.
7
Structural basis of histidine kinase autophosphorylation deduced by integrating genomics, molecular dynamics, and mutagenesis.通过整合基因组学、分子动力学和诱变,推断组氨酸激酶自身磷酸化的结构基础。
Proc Natl Acad Sci U S A. 2012 Jun 26;109(26):E1733-42. doi: 10.1073/pnas.1201301109. Epub 2012 Jun 5.
8
DEER distance measurements on proteins.蛋白质的双电子-电子共振距离测量。
Annu Rev Phys Chem. 2012;63:419-46. doi: 10.1146/annurev-physchem-032511-143716. Epub 2012 Jan 30.
9
Temperature-scan cryocrystallography reveals reaction intermediates in bacteriophytochrome.温度扫描低温晶体学揭示了细菌视紫红质中的反应中间体。
Nature. 2011 Oct 16;479(7373):428-32. doi: 10.1038/nature10506.
10
Rotamer libraries of spin labelled cysteines for protein studies.用于蛋白质研究的自旋标记半胱氨酸的构象文库。
Phys Chem Chem Phys. 2011 Feb 14;13(6):2356-66. doi: 10.1039/c0cp01865a. Epub 2010 Nov 30.

通过脉冲电子-电子双共振(PELDOR)测量不同自旋标记位置之间的全长二聚体细菌光敏色素Agp1的亚基间距离,在光转化后保持不变。

Intersubunit distances in full-length, dimeric, bacterial phytochrome Agp1, as measured by pulsed electron-electron double resonance (PELDOR) between different spin label positions, remain unchanged upon photoconversion.

作者信息

Kacprzak Sylwia, Njimona Ibrahim, Renz Anja, Feng Juan, Reijerse Edward, Lubitz Wolfgang, Krauss Norbert, Scheerer Patrick, Nagano Soshichiro, Lamparter Tilman, Weber Stefan

机构信息

From the Albert-Ludwigs-Universität Freiburg, Institut für Physikalische Chemie, 79104 Freiburg, Germany,

the Karlsruhe Institute of Technology, Botanical Institute I, 76131 Karlsruhe, Germany.

出版信息

J Biol Chem. 2017 May 5;292(18):7598-7606. doi: 10.1074/jbc.M116.761882. Epub 2017 Mar 13.

DOI:10.1074/jbc.M116.761882
PMID:28289094
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5418057/
Abstract

Bacterial phytochromes are dimeric light-regulated histidine kinases that convert red light into signaling events. Light absorption by the N-terminal photosensory core module (PCM) causes the proteins to switch between two spectrally distinct forms, Pr and Pfr, thus resulting in a conformational change that modulates the C-terminal histidine kinase region. To provide further insights into structural details of photoactivation, we investigated the full-length Agp1 bacteriophytochrome from the soil bacterium using a combined spectroscopic and modeling approach. We generated seven mutants suitable for spin labeling to enable application of pulsed EPR techniques. The distances between attached spin labels were measured using pulsed electron-electron double resonance spectroscopy to probe the arrangement of the subunits within the dimer. We found very good agreement of experimental and calculated distances for the histidine-kinase region when both subunits are in a parallel orientation. However, experimental distance distributions surprisingly showed only limited agreement with either parallel- or antiparallel-arranged dimer structures when spin labels were placed into the PCM region. This observation indicates that the arrangements of the PCM subunits in the full-length protein dimer in solution differ significantly from that in the PCM crystals. The pulsed electron-electron double resonance data presented here revealed either no or only minor changes of distance distributions upon Pr-to-Pfr photoconversion.

摘要

细菌光敏色素是二聚体光调节组氨酸激酶,可将红光转化为信号事件。N端光感受核心模块(PCM)对光的吸收会使蛋白质在两种光谱不同的形式Pr和Pfr之间转换,从而导致构象变化,进而调节C端组氨酸激酶区域。为了进一步深入了解光激活的结构细节,我们使用光谱学和建模相结合的方法研究了来自土壤细菌的全长Agp1细菌光敏色素。我们构建了七个适合自旋标记的突变体,以便应用脉冲电子顺磁共振技术。使用脉冲电子-电子双共振光谱测量附着的自旋标记之间的距离,以探测二聚体内亚基的排列。我们发现,当两个亚基呈平行方向时,组氨酸激酶区域的实验距离与计算距离非常吻合。然而,当自旋标记置于PCM区域时,实验距离分布令人惊讶地仅与平行或反平行排列的二聚体结构有有限的一致性。这一观察结果表明,溶液中全长蛋白质二聚体中PCM亚基的排列与PCM晶体中的排列有显著差异。本文给出的脉冲电子-电子双共振数据显示,在Pr到Pfr的光转换过程中,距离分布没有变化或只有微小变化。