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本文引用的文献

1
Cy3-DNA stacking interactions strongly depend on the identity of the terminal basepair.Cy3-DNA 堆积相互作用强烈依赖于末端碱基对的身份。
Biophys J. 2011 Feb 16;100(4):1049-57. doi: 10.1016/j.bpj.2011.01.014.
2
Cyanine dyes in biophysical research: the photophysics of polymethine fluorescent dyes in biomolecular environments.生物物理研究中的菁染料:生物分子环境中聚甲川荧光染料的光物理。
Q Rev Biophys. 2011 Feb;44(1):123-51. doi: 10.1017/S0033583510000247. Epub 2010 Nov 26.
3
The structure and folding of branched RNA analyzed by fluorescence resonance energy transfer.通过荧光共振能量转移分析分支RNA的结构与折叠。
Methods Enzymol. 2009;469:159-87. doi: 10.1016/S0076-6879(09)69008-X.
4
Photophysics of backbone fluorescent DNA modifications: reducing uncertainties in FRET.主链荧光DNA修饰的光物理:减少荧光共振能量转移中的不确定性
J Phys Chem B. 2009 Jun 4;113(22):7861-6. doi: 10.1021/jp810842u.
5
Nucleic acid base analog FRET-pair facilitating detailed structural measurements in nucleic acid containing systems.核酸碱基类似物荧光共振能量转移对有助于在含核酸系统中进行详细的结构测量。
J Am Chem Soc. 2009 Apr 1;131(12):4288-93. doi: 10.1021/ja806944w.
6
Nucleobase-specific enhancement of Cy3 fluorescence.胞嘧啶碱基对Cy3荧光的特异性增强。
J Fluoresc. 2009 May;19(3):443-8. doi: 10.1007/s10895-008-0431-1. Epub 2008 Oct 30.
7
Orientation dependence in fluorescent energy transfer between Cy3 and Cy5 terminally attached to double-stranded nucleic acids.与双链核酸末端相连的Cy3和Cy5之间荧光能量转移的方向依赖性
Proc Natl Acad Sci U S A. 2008 Aug 12;105(32):11176-81. doi: 10.1073/pnas.0801707105. Epub 2008 Aug 1.
8
The structure of cyanine 5 terminally attached to double-stranded DNA: implications for FRET studies.末端连接双链DNA的花青素5的结构:对荧光共振能量转移研究的启示。
Biochemistry. 2008 Jul 29;47(30):7857-62. doi: 10.1021/bi800773f. Epub 2008 Jul 3.
9
Advances in single-molecule fluorescence methods for molecular biology.用于分子生物学的单分子荧光方法进展
Annu Rev Biochem. 2008;77:51-76. doi: 10.1146/annurev.biochem.77.070606.101543.
10
Fluorescence properties and photophysics of the sulfoindocyanine Cy3 linked covalently to DNA.与DNA共价连接的磺化吲哚菁Cy3的荧光特性和光物理性质
J Phys Chem B. 2007 Sep 20;111(37):11064-74. doi: 10.1021/jp072912u. Epub 2007 Aug 24.

通过长而灵活的连接物将氰基荧光团末端连接到 DNA 上的定向。

Orientation of cyanine fluorophores terminally attached to DNA via long, flexible tethers.

机构信息

Cancer Research UK Nucleic Acid Structure Research Group, The University of Dundee, Dundee, United Kingdom.

出版信息

Biophys J. 2011 Sep 7;101(5):1148-54. doi: 10.1016/j.bpj.2011.07.007.

DOI:10.1016/j.bpj.2011.07.007
PMID:21889452
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3164170/
Abstract

Cyanine fluorophores are commonly used in single-molecule FRET experiments with nucleic acids. We have previously shown that indocarbocyanine fluorophores attached to the 5'-termini of DNA and RNA via three-carbon atom linkers stack on the ends of the helix, orienting their transition moments. We now investigate the orientation of sulfoindocarbocyanine fluorophores tethered to the 5'-termini of DNA via 13-atom linkers. Fluorescence lifetime measurements of sulfoindocarbocyanine 3 attached to double-stranded DNA indicate that the fluorophore is extensively stacked onto the terminal basepair at 15 °C, with properties that depend on the terminal sequence. In single molecules of duplex DNA, FRET efficiency between sulfoindocarbocyanine 3 and 5 attached in this manner is modulated with helix length, indicative of fluorophore orientation and consistent with stacked fluorophores that can undergo lateral motion. We conclude that terminal stacking is an intrinsic property of the cyanine fluorophores irrespective of the length of the tether and the presence or absence of sulfonyl groups. However, compared to short-tether indocarbocyanine, the mean rotational relationship between the two fluorophores is changed by ∼60° for the long-tether sulfoindocarbocyanine fluorophores. This is consistent with the transition moments becoming approximately aligned with the long axis of the terminal basepair for the long-linker species.

摘要

菁染料荧光团常用于核酸的单分子 FRET 实验。我们之前已经表明,通过三个碳原子链接器连接到 DNA 和 RNA 5'末端的吲哚菁染料荧光团堆积在螺旋的末端,使其跃迁矩定向。现在,我们研究了通过 13 个原子链接器连接到 DNA 5'末端的磺基吲哚菁染料荧光团的取向。磺基吲哚菁染料 3 与双链 DNA 结合的荧光寿命测量表明,在 15°C 时,荧光团广泛堆积在末端碱基对,其性质取决于末端序列。在双链 DNA 的单分子中,以这种方式连接的磺基吲哚菁染料 3 和 5 之间的 FRET 效率随螺旋长度而变化,表明荧光团的取向与可以进行横向运动的堆叠荧光团一致。我们得出结论,末端堆积是菁染料荧光团的固有特性,与链接的长度以及是否存在磺酰基无关。然而,与短链接的吲哚菁相比,对于长链接的磺基吲哚菁染料,两个荧光团之间的平均旋转关系发生了约 60°的变化。这与长链连接物物种的跃迁矩与末端碱基对的长轴大致对齐的情况一致。