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Total internal reflection fluorescence anisotropy imaging microscopy: setup calibration and data processing for protein polymerization measurements in living cells

机译:全内反射荧光各向异性成像显微镜:用于活细胞中蛋白质聚合测量的设置校准和数据处理

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摘要

Fluorescence anisotropy imaging microscopy (FAIM) measures the depolarization properties of fluorophores to deduce molecular changes in their environment. For successful FAIM, several design principles have to be considered and a thorough system-specific calibration protocol is paramount. One important calibration parameter is the G factor, which describes the system-induced errors for different polarization states of light. The determination and calibration of the G factor is discussed in detail in this article. We present a novel measurement strategy, which is particularly suitable for FAIM with high numerical aperture objectives operating in TIRF illumination mode. The method makes use of evanescent fields that excite the sample with a polarization direction perpendicular to the image plane. Furthermore, we have developed an ImageJ/Fiji plugin, AniCalc, for FAIM data processing. We demonstrate the capabilities of our TIRF-FAIM system by measuring β-actin polymerization in human embryonic kidney cells and in retinal neurons.
机译:荧光各向异性成像显微镜(FAIM)测量荧光团的去极化特性,以推断其环境中的分子变化。对于成功的FAIM,必须考虑多种设计原则,而全面的系统特定校准协议至关重要。一个重要的校准参数是G因子,它描述了系统针对不同偏振态的光引起的误差。本文将详细讨论G因子的确定和校准。我们提出了一种新颖的测量策略,该策略特别适用于在TIRF照明模式下运行的具有高数值孔径物镜的FAIM。该方法利用了消逝场,该消逝场以垂直于像平面的偏振方向激发样品。此外,我们还开发了用于FAIM数据处理的ImageJ / Fiji插件AniCalc。我们通过测量人类胚胎肾细胞和视网膜神经元中的β-肌动蛋白聚合来证明TIRF-FAIM系统的功能。

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