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首页> 外文期刊>Journal of Cell Science >Control of localization of a spindle checkpoint protein, Mad2, in fission yeast.
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Control of localization of a spindle checkpoint protein, Mad2, in fission yeast.

机译:裂变酵母中纺锤体检查点蛋白Mad2的定位控制。

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摘要

To ensure accurate chromosome segregation, the spindle checkpoint delays the onset of sister chromatid separation when the spindle is not attached to a kinetochore. Mad2, a component of the checkpoint, targets fission yeast Slp1/budding yeast Cdc20/human p55CDC and prevents it from promoting proteolysis, which is a prerequisite to sister chromatid separation. The protein is localized to unattached kinetochores in higher eukaryotes, and it is thought to be required for activation of the checkpoint as well. In this study, Mad2 and its target Slp1 were visualized in a tractable organism, fission yeast Schizosaccharomyces pombe. When cells were arrested at a prometaphase-like stage, the Mad2-Slp1 complex was stable and the two proteins were colocalized to unattached kinetochores. When the spindle attachment was completed, the complex was no longer detectable and only Mad2 was found associated to the spindle. These results would suggest that unattached kinetochores provide sites for assembly of the Mad2-Slp1 complex. During interphase, Mad2 was localized to the nuclear periphery as well as to the chromatin domain. This localization was abolished in a yeast strain lacking Mad1, a protein that physically interacts with Mad2. Mad1 may anchor Mad2 to the nuclear membrane and regulate its entry into the nucleus.
机译:为了确保准确的染色体分离,当纺锤体未连接到动粒上时,纺锤体检查点会延迟姐妹染色单体分离的开始。 Mad2是检查点的组成部分,其目标是裂变酵母Slp1 /萌芽酵母Cdc20 /人p55CDC并阻止其促进蛋白水解,这是姐妹染色单体分离的先决条件。该蛋白质定位于高等真核生物中独立的动植物,并且也被认为是激活检查点所必需的。在这项研究中,Mad2及其靶标Slp1在易裂变生物裂殖酵母粟酒裂殖酵母中可见。当细胞停滞在前中期样阶段时,Mad2-Slp1复合物是稳定的,并且这两种蛋白共定位于未连接的动植物。主轴连接完成后,复合体不再可检测,仅发现与主轴相关的Mad2。这些结果表明,独立的动植物提供了Mad2-Slp1复合体的组装位点。在相间期,Mad2定位于核外围以及染色质域。这种定位在缺少Mad1的酵母菌株中被取消了,Mad1是一种与Mad2发生物理相互作用的蛋白质。 Mad1可以将Mad2锚定在核膜上,并调节其进入核的过程。

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