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基于强度、光谱和寿命成像比较福斯特共振能量转移测量精度的量化

Comparing the quantification of Forster resonance energy transfer measurement accuracies based on intensity, spectral, and lifetime imaging.

作者信息

Pelet Serge, Previte Michael J R, So Peter T C

机构信息

Massachusetts Institute of Technology, Department of Mechanical Engineering, Cambridge, Massachusetts 02139, USA.

出版信息

J Biomed Opt. 2006 May-Jun;11(3):34017. doi: 10.1117/1.2203664.

Abstract

The measurement of Forster resonance energy transfer (FRET) in microscopes can be realized by different imaging modalities. In the present work, reference FRET constructs are developed to allow the comparison of FRET microscopy measurements using intensity, spectral, and lifetime imaging. Complimentary DNA strands are respectively labeled with Oregon Green 488 (OG488) or tetramethylrhodamine (TMR). The OG488 dye is fixed at the 5(') end of one strand, and the TMR label position is allowed to vary along the complimentary strand. Since OG488 and TMR are FRET pairs, the FRET efficiency can be determined theoretically from the distance separating the two dyes of the double-stranded DNA molecules. Microscopic images are formed by imaging microcapillaries containing various mixtures of oligonucleotides labeled with the FRET fluorophore pair, only the donor, or only acceptor. Traditional two-channel intensity measurements are compared with spectrally resolved imaging and fluorescence lifetime imaging by calculating a FRET index. The latter proves to be the best method to quantify FRET efficiency in the image. More importantly, the intensity fraction of molecules undergoing FRET can be quantitatively measured in each pixel of the image.

摘要

显微镜中福斯特共振能量转移(FRET)的测量可通过不同的成像方式实现。在本工作中,开发了参考FRET构建体,以比较使用强度、光谱和寿命成像的FRET显微镜测量。互补DNA链分别用俄勒冈绿488(OG488)或四甲基罗丹明(TMR)标记。OG488染料固定在一条链的5(')端,TMR标记位置可沿互补链变化。由于OG488和TMR是FRET对,理论上可根据双链DNA分子中两种染料之间的距离确定FRET效率。通过对含有用FRET荧光团对、仅供体或仅受体标记的寡核苷酸各种混合物的微毛细管成像来形成显微图像。通过计算FRET指数,将传统的双通道强度测量与光谱分辨成像和荧光寿命成像进行比较。结果证明,后者是量化图像中FRET效率的最佳方法。更重要的是,可在图像的每个像素中定量测量发生FRET的分子的强度分数。

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