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True emission and absorption anisotropies for the study of protein rotation obtained from fluorescence depletion measurements in various experimental geometries

机译:用于研究从各种实验几何形状中荧光耗尽测量获得的蛋白质旋转研究的真正排放和吸收各向异性

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The utility of fluorescence depletion methods for the measurement of slow protein rotational diffusion has been limited by the lack of a rigorous mathematical model to obtain, from depletion data, anisotropies directly comparable to those obtained from phosphorescence emission or triplet absorption measurements. A generalized theory to meet this need is described. The experimental method requires the acquisition of, at most, three separate measurements to calculate absorption or emission anisotropies. Each measurement is made with a different orientation of either the probe beam polarization, pump beam polarization, or emission polarizer. The results of the theory are applied to two experimental configurations. The first of these involves collecting emission at 90$DGR to colinear pump and probe beams. From such data we are able to calculate the absorption anisotropy, the emission anisotropy, and the interdipole angle. The second configuration represents a system where all polarization axes lie in a single plane as would occur in a microscope-based system. For this configuration we are able to calculate, given the interdipole angle derived from the 90$DGR case, the true absorption anisotropy, the true emission anisotropy, or both.
机译:荧光耗尽方法用于测量缓慢蛋白质旋转扩散的方法受到缺乏严格的数学模型,从耗尽数据中获得直接可与磷光发射或三重态吸收测量结果直接相当的各向异性。描述了满足这种需求的广义理论。实验方法需要最多三次单独测量来计算吸收或排放各向异性。通过探针偏振,泵束极化或发射偏振器的不同取向进行每个测量。该理论的结果应用于两种实验配置。其中的第一个涉及将90美元的发射收集到Colinear泵和探针梁。从这些数据中,我们能够计算吸收各向异性,发射各向异性和偶域角度。第二配置表示在基于显微镜的系统中发生的所有偏振轴位于单个平面中的系统。对于这种配置,我们能够计算出来自90美元DGR案例的偶极面积,真正的吸收各向异性,真正的排放各向异性或两者。

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