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Multiscale Analysis of Dynamics and Interactions of Heterochromatin Protein 1 by Fluorescence Fluctuation Microscopy

机译:荧光波动显微镜对异染色质蛋白1动力学和相互作用的多尺度分析

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摘要

Heterochromatin protein 1 (HP1) is a central factor in establishing and maintaining the repressive heterochromatin state. To elucidate its mobility and interactions, we conducted a comprehensive analysis on different time and length scales by fluorescence fluctuation microscopy in mouse cell lines. The local mobility of HP1α and HP1β was investigated in densely packed pericentric heterochromatin foci and compared with other bona fide euchromatin regions of the nucleus by fluorescence bleaching and correlation methods. A quantitative description of HP1α/β in terms of its concentration, diffusion coefficient, kinetic binding, and dissociation rate constants was derived. Three distinct classes of chromatin-binding sites with average residence times tres ≤ 0.2 s (class I, dominant in euchromatin), 7 s (class II, dominant in heterochromatin), and ∼2 min (class III, only in heterochromatin) were identified. HP1 was present at low micromolar concentrations at heterochromatin foci, and required histone H3 lysine 9 methylases Suv39h1/2 for two- to fourfold enrichment at these sites. These findings impose a number of constraints for the mechanism by which HP1 is able to maintain a heterochromatin state.
机译:异染色质蛋白1(HP1)是建立和维持阻抑异染色质状态的重要因素。为了阐明其移动性和相互作用,我们通过荧光波动显微镜在小鼠细胞系中对不同的时间和长度尺度进行了全面分析。 HP1α和HP1β的局部迁移率在密集堆积的外周中心异染色质病灶中进行了研究,并通过荧光漂白和相关方法将其与细胞核的其他真正染色质区进行了比较。得出了HP1α/β的浓度,扩散系数,动力学结合和解离速率常数的定量描述。鉴定出三类不同的染色质结合位点,其平均停留时间tres≤0.2 s(I类,在常染色质中占优势),7 s(II类,在异染色质中占优势)和约2分钟(III类,仅在异染色质中)。 。 HP1在异染色质的焦点处以低微摩尔浓度存在,并且需要组蛋白H3赖氨酸9甲基化酶Suv39h1 / 2才能在这些位点富集2至4倍。这些发现对HP1能够维持异染色质状态的机制施加了许多限制。

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