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Mapping eGFP Oligomer Mobility in Living Cell Nuclei

机译:映射活细胞核中的eGFP低聚物运动性

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摘要

Movement of particles in cell nuclei can be affected by viscosity, directed flows, active transport, or the presence of obstacles such as the chromatin network. Here we investigate whether the mobility of small fluorescent proteins is affected by the chromatin density. Diffusion of inert fluorescent proteins was studied in living cell nuclei using fluorescence correlation spectroscopy (FCS) with a two-color confocal scanning detection system. We first present experiments exposing FCS-specific artifacts encountered in live cell studies as well as strategies to prevent them, in particular those arising from the choice of the fluorophore used for calibration of the focal volume, as well as temperature and acquisition conditions used for fluorescence fluctuation measurements. After defining the best acquisition conditions, we show for various human cell lines that the mobility of GFP varies significantly within the cell nucleus, but does not correlate with chromatin density. The intranuclear diffusional mobility strongly depends on protein size: in a series of GFP-oligomers, used as free inert fluorescent tracers, the diffusion coefficient decreased from the monomer to the tetramer much more than expected for molecules free in aqueous solution. Still, the entire intranuclear chromatin network is freely accessible for small proteins up to the size of eGFP-tetramers, regardless of the chromatin density or cell line. Even the densest chromatin regions do not exclude free eGFP-monomers or multimers.
机译:颗粒在细胞核中的移动可能会受到粘度,定向流动,主动转运或存在诸如染色质网络之类的障碍物的影响。在这里我们调查小的荧光蛋白的迁移率是否受染色质密度的影响。惰性荧光蛋白在活细胞核中的扩散通过使用荧光相关光谱法(FCS)和双色共聚焦扫描检测系统进行了研究。我们首先介绍的实验揭示了活细胞研究中遇到的FCS特有的伪影及其预防策略,特别是那些由于选择用于校准焦距的荧光团以及用于荧光的温度和采集条件而产生的伪影波动测量。定义最佳的采集条件后,我们显示出对于各种人类细胞系,GFP的迁移率在细胞核内显着变化,但与染色质密度无关。核内扩散迁移率在很大程度上取决于蛋白质的大小:在用作自由惰性荧光示踪剂的一系列GFP-寡聚物中,从单体到四聚体的扩散系数下降的幅度远远大于水溶液中游离分子的预期。尽管如此,无论染色质密度或细胞系如何,整个小分子蛋白都可以自由访问整个核内染色质网络,直到eGFP-四聚体的大小。即使最密集的染色质区域也不排除游离的eGFP单体或多聚体。

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