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出芽酵母Tem1p、Cdc15p和Bub2p蛋白动力学在有丝分裂退出中的不同作用。

The differential roles of budding yeast Tem1p, Cdc15p, and Bub2p protein dynamics in mitotic exit.

作者信息

Molk Jeffrey N, Schuyler Scott C, Liu Jenny Y, Evans James G, Salmon E D, Pellman David, Bloom Kerry

机构信息

Department of Biology, University of North Carolina, Chapel Hill, North Carolina 27599, USA.

出版信息

Mol Biol Cell. 2004 Apr;15(4):1519-32. doi: 10.1091/mbc.e03-09-0708. Epub 2004 Jan 12.

Abstract

In the budding yeast Saccharomyces cerevisiae the mitotic spindle must be positioned along the mother-bud axis to activate the mitotic exit network (MEN) in anaphase. To examine MEN proteins during mitotic exit, we imaged the MEN activators Tem1p and Cdc15p and the MEN regulator Bub2p in vivo. Quantitative live cell fluorescence microscopy demonstrated the spindle pole body that segregated into the daughter cell (dSPB) signaled mitotic exit upon penetration into the bud. Activation of mitotic exit was associated with an increased abundance of Tem1p-GFP and the localization of Cdc15p-GFP on the dSPB. In contrast, Bub2p-GFP fluorescence intensity decreased in mid-to-late anaphase on the dSPB. Therefore, MEN protein localization fluctuates to switch from Bub2p inhibition of mitotic exit to Cdc15p activation of mitotic exit. The mechanism that elevates Tem1p-GFP abundance in anaphase is specific to dSPB penetration into the bud and Dhc1p and Lte1p promote Tem1p-GFP localization. Finally, fluorescence recovery after photobleaching (FRAP) measurements revealed Tem1p-GFP is dynamic at the dSPB in late anaphase. These data suggest spindle pole penetration into the bud activates mitotic exit, resulting in Tem1p and Cdc15p persistence at the dSPB to initiate the MEN signal cascade.

摘要

在出芽酵母酿酒酵母中,有丝分裂纺锤体必须沿母细胞 - 芽轴定位,以便在后期激活有丝分裂退出网络(MEN)。为了在有丝分裂退出过程中检测MEN蛋白,我们在体内对MEN激活因子Tem1p和Cdc15p以及MEN调节因子Bub2p进行了成像。定量活细胞荧光显微镜显示,分离到子细胞中的纺锤体极体(dSPB)在进入芽体时发出有丝分裂退出信号。有丝分裂退出的激活与Tem1p - GFP丰度的增加以及Cdc15p - GFP在dSPB上的定位有关。相比之下,在后期中期到后期,dSPB上的Bub2p - GFP荧光强度降低。因此,MEN蛋白的定位发生波动,从Bub2p对有丝分裂退出的抑制转变为Cdc15p对有丝分裂退出的激活。后期提高Tem1p - GFP丰度的机制特定于dSPB进入芽体,并且Dhc1p和Lte1p促进Tem1p - GFP的定位。最后,光漂白后荧光恢复(FRAP)测量显示,后期晚期Tem1p - GFP在dSPB处是动态的。这些数据表明纺锤体极体进入芽体激活有丝分裂退出,导致Tem1p和Cdc15p在dSPB处持续存在以启动MEN信号级联反应。

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