首页> 美国卫生研究院文献>The Journal of Biophysical and Biochemical Cytology >Interphase Cell Cycle Dynamics of a Late-Replicating Heterochromatic Homogeneously Staining Region: Precise Choreography of Condensation/Decondensation and Nuclear Positioning
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Interphase Cell Cycle Dynamics of a Late-Replicating Heterochromatic Homogeneously Staining Region: Precise Choreography of Condensation/Decondensation and Nuclear Positioning

机译:后期复制异色均质染色区域的相间细胞周期动力学:冷凝/去冷凝和核定位的精确编排。

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摘要

Recently we described a new method for in situ localization of specific DNA sequences, based on lac operator/repressor recognition (Robinett, C.C., A. Straight, G. Li, C. Willhelm, G. Sudlow, A. Murray, and A.S. Belmont. 1996. J. Cell Biol. 135:1685–1700). We have applied this methodology to visualize the cell cycle dynamics of an ∼90 Mbp, late-replicating, heterochromatic homogeneously staining region (HSR) in CHO cells, combining immunostaining with direct in vivo observations. Between anaphase and early G1, the HSR extends approximately twofold to a linear, ∼0.3-μm-diam chromatid, and then recondenses to a compact mass adjacent to the nuclear envelope. No further changes in HSR conformation or position are seen through mid-S phase. However, HSR DNA replication is preceded by a decondensation and movement of the HSR into the nuclear interior 4–6 h into S phase. During DNA replication the HSR resolves into linear chromatids and then recondenses into a compact mass; this is followed by a third extension of the HSR during G2/ prophase. Surprisingly, compaction of the HSR is extremely high at all stages of interphase. Preliminary ultrastructural analysis of the HSR suggests at least three levels of large-scale chromatin organization above the 30-nm fiber.
机译:最近,我们描述了一种基于lac操纵子/阻遏物识别的特定DNA序列原位定位的新方法(Robinett,CC,A。Straight,G。Li,C。Willhelm,G。Sudlow,A。Murray和AS Belmont 1996.J.Cell Biol.135:1685-1700)。我们已经应用了这种方法来可视化CHO细胞中约90 Mbp的,后期复制的异色均质染色区(HSR)的细胞周期动态,并结合了直接体内观察的免疫染色。在后期和G1早期之间,HSR延伸大约两倍,形成一个线性的,直径约为0.3μm的染色质,然后再凝结成一个紧密的核团。在S中期,没有看到高铁构象或位置的进一步变化。但是,在高铁DNA复制之前,高铁会发生缩聚,并在4-6小时内进入S相进入核内。在DNA复制过程中,HSR解析为线性染色单体,然后再浓缩成紧密的团块。这是在G2 /前期HSR的第三次延伸。出乎意料的是,在相间的所有阶段,高铁的压实度都非常高。 HSR的初步超微结构分析表明,在30 nm光纤上方,至少有三个水平的大规模染色质组织。

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