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端粒的实时成像:yKu和Sir蛋白在酵母中定义了冗余的端粒锚定途径。

Live imaging of telomeres: yKu and Sir proteins define redundant telomere-anchoring pathways in yeast.

作者信息

Hediger Florence, Neumann Frank R, Van Houwe Griet, Dubrana Karine, Gasser Susan M

机构信息

University of Geneva, Department of Molecular Biology, Quai Ernest-Ansermet 30, CH-1211 Geneva 4, Switzerland.

出版信息

Curr Biol. 2002 Dec 23;12(24):2076-89. doi: 10.1016/s0960-9822(02)01338-6.

Abstract

BACKGROUND

The positioning of chromosomal domains within interphase nuclei is thought to facilitate transcriptional repression in yeast. Although this is particularly well characterized for telomeres, the molecular basis of their specific subnuclear organization is poorly understood. The use of live fluorescence imaging overcomes limitations of in situ staining on fixed cells and permits the analysis of chromatin dynamics in relation to stages of the cell cycle.

RESULTS

We have characterized the dynamics of yeast telomeres and their associated domains of silent chromatin by using rapid time-lapse microscopy. In interphase, native telomeres are highly dynamic but remain within a restricted volume adjacent to the nuclear envelope. This constraint is lost during mitosis. A quantitative analysis of selected mutants shows that the yKu complex is necessary for anchoring some telomeres at the nuclear envelope (NE), whereas the myosin-like proteins Mlp1 and Mlp2 are not. We are able to correlate increased telomeric repression with increased anchoring and show that silent chromatin is tethered to the NE in a Sir-dependent manner in the absence of the yKu complex. Sir-mediated anchoring is S phase specific, while the yKu-mediated pathway functions throughout interphase. Subtelomeric elements of yeast telomere structure influence the relative importance of the yKu- and Sir-dependent mechanisms.

CONCLUSIONS

Interphase positioning of telomeres can be achieved through two partially redundant mechanisms. One requires the heterodimeric yKu complex, but not Mlp1 and Mlp2. The second requires Silent information regulators, correlates with transcriptional repression, and is specific to S phase.

摘要

背景

间期细胞核内染色体结构域的定位被认为有助于酵母中的转录抑制。尽管端粒的这一特性已得到充分表征,但其特定亚核组织的分子基础仍知之甚少。实时荧光成像克服了固定细胞原位染色的局限性,并允许分析与细胞周期阶段相关的染色质动力学。

结果

我们通过使用快速延时显微镜对酵母端粒及其相关的沉默染色质结构域的动力学进行了表征。在间期,天然端粒高度动态,但仍保留在靠近核膜的受限体积内。这种限制在有丝分裂期间消失。对选定突变体的定量分析表明,yKu复合物对于将一些端粒锚定在核膜(NE)上是必需的,而肌球蛋白样蛋白Mlp1和Mlp2则不是。我们能够将端粒抑制的增加与锚定的增加相关联,并表明在没有yKu复合物的情况下,沉默染色质以Sir依赖的方式与NE相连。Sir介导的锚定是S期特异性的,而yKu介导的途径在整个间期都起作用。酵母端粒结构的亚端粒元件影响yKu和Sir依赖机制的相对重要性。

结论

端粒的间期定位可以通过两种部分冗余的机制实现。一种需要异二聚体yKu复合物,但不需要Mlp1和Mlp2。第二种需要沉默信息调节因子,与转录抑制相关,并且是S期特异性的。

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