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首页> 外文期刊>BMC Cell Biology >4-D single particle tracking of synthetic and proteinaceous microspheres reveals preferential movement of nuclear particles along chromatin – poor tracks
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4-D single particle tracking of synthetic and proteinaceous microspheres reveals preferential movement of nuclear particles along chromatin – poor tracks

机译:合成和蛋白质微球的4-D单粒子跟踪揭示了核粒子沿染色质的优先运动-不良轨迹

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Background The dynamics of nuclear organization, nuclear bodies and RNPs in particular has been the focus of many studies. To understand their function, knowledge of their spatial nuclear position and temporal translocation is essential. Typically, such studies generate a wealth of data that require novel methods in image analysis and computational tools to quantitatively track particle movement on the background of moving cells and shape changing nuclei. Results We developed a novel 4-D image processing platform (TIKAL) for the work with laser scanning and wide field microscopes. TIKAL provides a registration software for correcting global movements and local deformations of cells as well as 2-D and 3-D tracking software. With this new tool, we studied the dynamics of two different types of nuclear particles, namely nuclear bodies made from GFP-NLS-vimentin and microinjected 0.1 μm – wide polystyrene beads, by live cell time-lapse microscopy combined with single particle tracking and mobility analysis. We now provide a tool for the automatic 3-D analysis of particle movement in parallel with the acquisition of chromatin density data. Conclusions Kinetic analysis revealed 4 modes of movement: confined obstructed, normal diffusion and directed motion. Particle tracking on the background of stained chromatin revealed that particle movement is directly related to local reorganization of chromatin. Further a direct comparison of particle movement in the nucleoplasm and the cytoplasm exhibited an entirely different kinetic behaviour of vimentin particles in both compartments. The kinetics of nuclear particles were slightly affected by depletion of ATP and significantly disturbed by disruption of actin and microtubule networks. Moreover, the hydration state of the nucleus had a strong impact on the mobility of nuclear bodies since both normal diffusion and directed motion were entirely abolished when cells were challenged with 0.6 M sorbitol. This effect correlated with the compaction of chromatin. We conclude that alteration in chromatin density directly influences the mobility of protein assemblies within the nucleus.
机译:背景技术核组织,特别是核机构和RNP的动态一直是许多研究的重点。要了解它们的功能,必须了解其空间核位置和时间易位。通常,此类研究会生成大量数据,这些数据需要图像分析和计算工具中的新颖方法来定量地跟踪运动细胞和形变核背景下的粒子运动。结果我们开发了一种新颖的4-D图像处理平台(TIKAL),可用于激光扫描和宽视场显微镜。 TIKAL提供了用于校正细胞整体运动和局部变形的注册软件,以及2-D和3-D跟踪软件。使用这个新工具,我们通过活细胞延时显微镜结合单粒子跟踪和迁移率研究了两种不同类型的核粒子的动力学,即由GFP-NLS-波形蛋白制成的核体和微注射的0.1μm宽聚苯乙烯珠。分析。现在,我们提供了一种工具,可在进行染色质密度数据采集的同时自动进行粒子运动的3-D分析。结论动力学分析揭示了四种运动模式:受限阻塞,正常扩散和定向运动。在染色质染色质背景上进行颗粒跟踪显示,颗粒运动与染色质的局部重组直接相关。进一步直接比较核质和细胞质中颗粒运动在两个区室中显示波形蛋白颗粒完全不同的动力学行为。 ATP的消耗对核颗粒的动力学影响很小,而肌动蛋白和微管网络的破坏则明显干扰核颗粒的动力学。而且,当细胞受到0.6 M山梨糖醇攻击时,正常的扩散和定向运动都被完全消除了,原子核的水合状态对核体的移动性产生了很大的影响。这种作用与染色质的压实有关。我们得出结论,染色质密度的改变直接影响细胞核内蛋白质装配体的迁移率。

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