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活细胞中DNA的直接成像揭示了染色体形成的动态过程。

Direct imaging of DNA in living cells reveals the dynamics of chromosome formation.

作者信息

Manders E M, Kimura H, Cook P R

机构信息

Sir William Dunn School of Pathology, University of Oxford, Oxford, OX1 3RE, United Kingdom.

出版信息

J Cell Biol. 1999 Mar 8;144(5):813-21. doi: 10.1083/jcb.144.5.813.

Abstract

Individual chromosomes are not directly visible within the interphase nuclei of most somatic cells; they can only be seen during mitosis. We have developed a method that allows DNA strands to be observed directly in living cells, and we use it to analyze how mitotic chromosomes form. A fluorescent analogue (e.g., Cy5-dUTP) of the natural precursor, thymidine triphosphate, is introduced into cells, which are then grown on the heated stage of a confocal microscope. The analogue is incorporated by the endogenous enzymes into DNA. As the mechanisms for recognizing and removing the unusual residues do not prevent subsequent progress around the cell cycle, the now fluorescent DNA strands can be followed as they assemble into chromosomes, and segregate to daughters and granddaughters. Movies of such strands in living cells suggest that chromosome axes follow simple recognizable paths through their territories during G2 phase, and that late replicating regions maintain their relative positions as prophase chromosomes form. Quantitative analysis confirms that individual regions move little during this stage of chromosome condensation. As a result, the gross structure of an interphase chromosome territory is directly related to that of the prophase chromosome.

摘要

在大多数体细胞的间期核内,单个染色体是不可直接见的;只有在有丝分裂期间才能看到它们。我们开发了一种方法,可直接在活细胞中观察DNA链,并利用该方法分析有丝分裂染色体的形成过程。将天然前体三磷酸胸苷的荧光类似物(如Cy5-dUTP)导入细胞,然后将细胞置于共聚焦显微镜的加热载物台上培养。该类似物被内源性酶掺入DNA中。由于识别和去除异常残基的机制并不妨碍细胞周期的后续进程,因此现在可以追踪荧光DNA链组装成染色体并分离到子细胞和孙细胞的过程。活细胞中此类DNA链的成像表明,染色体轴在G2期通过其所在区域遵循简单可识别的路径,并且在前期染色体形成时,晚复制区域保持其相对位置。定量分析证实,在染色体凝聚的这个阶段,各个区域移动很少。因此,间期染色体区域的总体结构与前期染色体的结构直接相关。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/54ff/2148202/a52e0012a576/JCB9809130.f1.jpg

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