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Imaging of fluorescence anisotropy during photoswitching provides a simple readout for protein self-association

机译:在照相机期间的荧光各向异性的成像提供了一种简单的蛋白质自我会读数

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Monitoring of protein oligomerization has benefited greatly from F?rster Resonance Energy Transfer (FRET) measurements. Although donors and acceptors are typically fluorescent molecules with different spectra, homo-FRET can occur between fluorescent molecules of the same type if the emission spectrum overlaps with the absorption spectrum. Here, we describe homo-FRET measurements by monitoring anisotropy changes in photoswitchable fluorescent proteins while photoswitching to the off state. These offer the capability to estimate anisotropy in the same specimen during homo-FRET as well as non-FRET conditions. We demonstrate photoswitching anisotropy FRET (psAFRET) with a number of test chimeras and example oligomeric complexes inside living cells. We also present an equation derived from FRET and anisotropy equations which converts anisotropy changes into a factor we call delta r FRET (drFRET). This is analogous to an energy transfer efficiency and allows experiments performed on a given homo-FRET pair to be more easily compared across different optical configurations.
机译:蛋白质低聚的监测从F?奔跑共振能量转移(FRET)测量中受益匪浅。虽然供体和受体通常是具有不同光谱的荧光分子,但如果发射光谱与吸收光谱重叠,则可以在相同类型的荧光分子之间发生同源物。在这里,我们通过监测光学荧光蛋白的各向异性变化,在光学开关到关闭状态时,通过监测各向异性变化来描述同性恋测量。这些能够在同住摩托车期间和非尺寸条件下估计同一样品中的各向异性。我们展示了具有多种试验嵌合体和外阴物细胞的低聚复合物的光学开关的各向异性FRET(PSAFRET)。我们还介绍了衍生自FRET的等式和各向异性方程,其将各向异性变化转换为呼叫DELTA R FRET(DRFRET)的因子。这类似于能量传递效率,并且允许在不同的光学配置中更容易地更容易地在给定的同性全面对上进行的实验。

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