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转录因子RUNX1/AML1和RUNX2/Cbfa1与静止的亚核结构域动态关联。

Transcription factors RUNX1/AML1 and RUNX2/Cbfa1 dynamically associate with stationary subnuclear domains.

作者信息

Harrington Kimberly S, Javed Amjad, Drissi Hicham, McNeil Sandra, Lian Jane B, Stein Janet L, Van Wijnen André J, Wang Yu-Li, Stein Gary S

机构信息

Department of Cell Biology and Cancer Center, University of Massachusetts Medical School, Worcester, Massachusetts 01655-0106, USA.

出版信息

J Cell Sci. 2002 Nov 1;115(Pt 21):4167-76. doi: 10.1242/jcs.00095.

Abstract

The runt-related transcription factors (RUNX/Cbfa/AML) are essential for cellular differentiation and fetal development. C-terminal truncations of RUNX factors that eliminate the targeting of these factors to subnuclear foci result in lethal hematopoietic and skeletal phenotypes. Here we demonstrate that in living cells the RUNX C-terminus is necessary for the dynamic association of RUNX into stable subnuclear domains. Time-lapse fluorescence microscopy shows that RUNX1 and RUNX2 localize to punctate foci that remain stationary in the nuclear space. By fluorescence recovery after photobleaching assays, both proteins are shown to dynamically associate at these subnuclear foci, with a 10 second half-time of recovery. A truncation of RUNX2, removing its intranuclear targeting signal (NMTS), increases its mobility by an order of magnitude, resulting in a half-time of recovery equivalent to that of EGFP alone. We propose that the dynamic shuttling of RUNX factors in living cells to positionally stabilized foci, which is dependent on the C-terminus, is a component of the mechanism for gene regulation in vivo.

摘要

与矮小相关的转录因子(RUNX/Cbfa/AML)对于细胞分化和胎儿发育至关重要。RUNX因子的C末端截短会消除这些因子定位于核内亚结构域的能力,从而导致致命的造血和骨骼表型。在此,我们证明在活细胞中,RUNX的C末端对于RUNX动态结合到稳定的核内亚结构域是必需的。延时荧光显微镜显示,RUNX1和RUNX2定位于核空间中保持静止的点状亚结构域。通过光漂白后荧光恢复分析表明,这两种蛋白在这些核内亚结构域动态结合,恢复半衰期为10秒。RUNX2的截短形式去除了其核内靶向信号(NMTS),使其迁移率增加了一个数量级,导致恢复半衰期与单独的增强绿色荧光蛋白(EGFP)相当。我们提出,活细胞中RUNX因子向位置稳定的亚结构域的动态穿梭,这依赖于C末端,是体内基因调控机制的一个组成部分。

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