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本文引用的文献

1
Raman spectroscopy reveals direct chromophore interactions in the Leu/Gln105 spectral tuning switch of proteorhodopsins.拉曼光谱揭示了视紫质蛋白Leu/Gln105光谱调谐开关中发色团的直接相互作用。
J Phys Chem B. 2008 Sep 18;112(37):11770-6. doi: 10.1021/jp802629e. Epub 2008 Aug 22.
2
Protonation state of Glu142 differs in the green- and blue-absorbing variants of proteorhodopsin.在视紫质的绿色吸收和蓝色吸收变体中,谷氨酸142的质子化状态有所不同。
Biochemistry. 2008 Mar 18;47(11):3447-53. doi: 10.1021/bi7018964. Epub 2008 Feb 20.
3
Subpicosecond protein backbone changes detected during the green-absorbing proteorhodopsin primary photoreaction.在绿色吸收型视紫红质初级光反应过程中检测到的亚皮秒级蛋白质主链变化。
J Phys Chem B. 2007 Oct 11;111(40):11824-31. doi: 10.1021/jp073490r. Epub 2007 Sep 19.
4
FTIR study of the retinal Schiff base and internal water molecules of proteorhodopsin.视紫红质的视网膜席夫碱和内部水分子的傅里叶变换红外光谱研究。
Biochemistry. 2007 May 8;46(18):5365-73. doi: 10.1021/bi700143g. Epub 2007 Apr 12.
5
The Sorcerer II Global Ocean Sampling expedition: northwest Atlantic through eastern tropical Pacific.“魔法师二号”全球海洋采样探险:从西北大西洋到东热带太平洋
PLoS Biol. 2007 Mar;5(3):e77. doi: 10.1371/journal.pbio.0050077.
6
Time-resolved FTIR spectroscopy of the photointermediates involved in fast transient H+ release by proteorhodopsin.对参与视紫质快速瞬态释放氢离子过程的光中间体进行时间分辨傅里叶变换红外光谱分析。
J Phys Chem B. 2005 Jan 13;109(1):634-41. doi: 10.1021/jp046314g.
7
Structure, function, and wavelength selection in blue-absorbing proteorhodopsin.吸收蓝光的视紫红质的结构、功能及波长选择
Biochemistry. 2006 Feb 14;45(6):1579-90. doi: 10.1021/bi051851s.
8
Functional waters in intraprotein proton transfer monitored by FTIR difference spectroscopy.傅里叶变换红外差示光谱法监测蛋白质内质子转移中的功能水。
Nature. 2006 Jan 5;439(7072):109-12. doi: 10.1038/nature04231. Epub 2005 Nov 9.
9
New insights into metabolic properties of marine bacteria encoding proteorhodopsins.对编码视紫红质的海洋细菌代谢特性的新见解。
PLoS Biol. 2005 Aug;3(8):e273. doi: 10.1371/journal.pbio.0030273. Epub 2005 Jul 19.
10
FTIR studies of internal water molecules in the Schiff base region of bacteriorhodopsin.细菌视紫红质席夫碱区域内水分子的傅里叶变换红外光谱研究。
Biochemistry. 2005 May 24;44(20):7406-13. doi: 10.1021/bi050122+.

在初级光反应过程中,蓝光视紫红质和绿光视紫红质会发生不同的结构变化。

Different structural changes occur in blue- and green-proteorhodopsins during the primary photoreaction.

作者信息

Amsden Jason J, Kralj Joel M, Bergo Vladislav B, Spudich Elena N, Spudich John L, Rothschild Kenneth J

机构信息

Department of Physics, Photonics Center, and Molecular Biophysics Laboratory, Boston University, Boston, Massachusetts 02215, USA.

出版信息

Biochemistry. 2008 Nov 4;47(44):11490-8. doi: 10.1021/bi800945t. Epub 2008 Oct 9.

DOI:10.1021/bi800945t
PMID:18842006
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3631532/
Abstract

We examine the structural changes during the primary photoreaction in blue-absorbing proteorhodopsin (BPR), a light-driven retinylidene proton pump, using low-temperature FTIR difference spectroscopy. Comparison of the light-induced BPR difference spectrum recorded at 80 K to that of green-absorbing proteorhodopsin (GPR) reveals that there are several differences in the BPR and GPR primary photoreactions despite the similar structure of the retinal chromophore and all-trans --> 13-cis isomerization. Strong bands near 1700 cm(-1) assigned previously to a change in hydrogen bonding of Asn230 in GPR are still present in BPR. However, additional bands in the same region are assigned on the basis of site-directed mutagenesis to changes occurring in Gln105. In the amide II region, bands are assigned on the basis of total (15)N labeling to structural changes of the protein backbone, although no such bands were previously observed for GPR. A band at 3642 cm(-1) in BPR, assigned to the OH stretching mode of a water molecule on the basis of H2(18)O substitution, appears at a different frequency than a band at 3626 cm(-1) previously assigned to a water molecule in GPR. However, the substitution of Gln105 for Leu105 in BPR leads to the appearance of both bands at 3642 and 3626 cm(-1), indicating the waters assigned in BPR and GPR exist in separate distinct locations and can coexist in the GPR-like Q105L mutant of BPR. These results indicate that there exist significant differences in the conformational changes occurring in these two types proteorhodopsin during the initial photoreaction despite their similar chromophore structures, which might reflect a different arrangement of water in the active site as well as substitution of a hydrophilic for hydrophobic residue at residue 105.

摘要

我们使用低温傅里叶变换红外差光谱法,研究了蓝光吸收型视黄醛质子泵——嗜盐菌视紫红质(BPR)初级光反应过程中的结构变化。将在80K下记录的光诱导BPR差光谱与绿光吸收型嗜盐菌视紫红质(GPR)的差光谱进行比较,结果表明,尽管视网膜发色团结构相似且都发生了全反式向13-顺式的异构化,但BPR和GPR的初级光反应仍存在若干差异。先前在GPR中归属于Asn230氢键变化的1700 cm⁻¹附近的强吸收带,在BPR中仍然存在。然而,基于定点诱变,同一区域的其他吸收带被归属于Gln105发生的变化。在酰胺II区域,基于全¹⁵N标记,吸收带被归属于蛋白质主链的结构变化,尽管先前在GPR中未观察到此类吸收带。基于H₂¹⁸O取代,BPR中3642 cm⁻¹处的吸收带被归属于水分子的OH伸缩模式,其出现的频率与先前在GPR中归属于水分子的3626 cm⁻¹处的吸收带不同。然而,BPR中Gln105被Leu105取代会导致3642和3626 cm⁻¹处都出现吸收带,这表明BPR和GPR中归属于水的位置是分开且不同的,并且可以在BPR的GPR样Q105L突变体中共存。这些结果表明,尽管这两种嗜盐菌视紫红质的发色团结构相似,但在初始光反应过程中发生的构象变化存在显著差异,这可能反映了活性位点中水的排列不同以及105位残基处亲水性残基被疏水性残基取代的情况。