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本文引用的文献

1
The budding yeast Ipl1/Aurora protein kinase regulates mitotic spindle disassembly.出芽酵母Ipl1/极光蛋白激酶调节有丝分裂纺锤体的解体。
J Cell Biol. 2003 Feb 3;160(3):329-39. doi: 10.1083/jcb.200209018.
2
Phospho-regulation of kinetochore-microtubule attachments by the Aurora kinase Ipl1p.极光激酶Ipl1p对动粒-微管附着的磷酸化调控
Cell. 2002 Oct 18;111(2):163-72. doi: 10.1016/s0092-8674(02)00973-x.
3
Chromosome dynamics: new light on Aurora B kinase function.染色体动力学:极光激酶B功能的新见解
Curr Biol. 2002 Jul 9;12(13):R458-60. doi: 10.1016/s0960-9822(02)00945-4.
4
Simple centromere, complex kinetochore: linking spindle microtubules and centromeric DNA in budding yeast.简单的着丝粒,复杂的动粒:在芽殖酵母中连接纺锤体微管和着丝粒DNA
J Cell Biol. 2002 Apr 15;157(2):199-203. doi: 10.1083/jcb.200201052.
5
Evidence that the Ipl1-Sli15 (Aurora kinase-INCENP) complex promotes chromosome bi-orientation by altering kinetochore-spindle pole connections.有证据表明Ipl1-Sli15(极光激酶-内着丝粒蛋白复合体)通过改变动粒-纺锤体极连接来促进染色体双定向。
Cell. 2002 Feb 8;108(3):317-29. doi: 10.1016/s0092-8674(02)00633-5.
6
The mitotic spindle is required for loading of the DASH complex onto the kinetochore.有丝分裂纺锤体是将DASH复合体加载到动粒上所必需的。
Genes Dev. 2002 Jan 15;16(2):183-97. doi: 10.1101/gad.959402.
7
Four new subunits of the Dam1-Duo1 complex reveal novel functions in sister kinetochore biorientation.Dam1-Duo1复合体的四个新亚基揭示了姐妹动粒双定向中的新功能。
EMBO J. 2002 Jan 15;21(1-2):181-93. doi: 10.1093/emboj/21.1.181.
8
Implication of a novel multiprotein Dam1p complex in outer kinetochore function.一种新型多蛋白Dam1p复合物在外着丝粒功能中的作用
J Cell Biol. 2001 Dec 24;155(7):1137-45. doi: 10.1083/jcb.200109063.
9
Systematic genetic analysis with ordered arrays of yeast deletion mutants.利用酵母缺失突变体有序阵列进行系统遗传分析。
Science. 2001 Dec 14;294(5550):2364-8. doi: 10.1126/science.1065810.
10
Functional cooperation of Dam1, Ipl1, and the inner centromere protein (INCENP)-related protein Sli15 during chromosome segregation.Dam1、Ipl1与着丝粒内蛋白(INCENP)相关蛋白Sli15在染色体分离过程中的功能协作。
J Cell Biol. 2001 Nov 26;155(5):763-74. doi: 10.1083/jcb.200105029.

动粒蛋白相互作用及其受极光激酶Ipl1p的调控

Kinetochore protein interactions and their regulation by the Aurora kinase Ipl1p.

作者信息

Shang Ching, Hazbun Tony R, Cheeseman Iain M, Aranda Jennifer, Fields Stanley, Drubin David G, Barnes Georjana

机构信息

Department of Molecular and Cell Biology, University of California, Berkeley, California 94720-3202, USA.

出版信息

Mol Biol Cell. 2003 Aug;14(8):3342-55. doi: 10.1091/mbc.e02-11-0765. Epub 2003 May 3.

DOI:10.1091/mbc.e02-11-0765
PMID:12925767
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC181571/
Abstract

Although there has been a recent explosion in the identification of budding yeast kinetochore components, the physical interactions that underlie kinetochore function remain obscure. To better understand how kinetochores attach to microtubules and how this attachment is regulated, we sought to characterize the interactions among kinetochore proteins, especially with respect to the microtubule-binding Dam1 complex. The Dam1 complex plays a crucial role in the chromosome-spindle attachment and is a key target for phospho-regulation of this attachment by the Aurora kinase Ipl1p. To identify protein-protein interactions involving the Dam1 complex, and the effects of Dam1p phosphorylation state on these physical interactions, we conducted both a genome-wide two-hybrid screen and a series of biochemical binding assays for Dam1p. A two-hybrid screen of a library of 6000 yeast open reading frames identified nine kinetochore proteins as Dam1p-interacting partners. From 113 in vitro binding reactions involving all nine subunits of the Dam1 complex and 32 kinetochore proteins, we found at least nine interactions within the Dam1 complex and 19 potential partners for the Dam1 complex. Strikingly, we found that the Dam1p-Ndc80p and Dam1p-Spc34p interactions were weakened by mutations mimicking phosphorylation at Ipl1p sites, allowing us to formulate a model for the effects of phosphoregulation on kinetochore function.

摘要

尽管最近在出芽酵母动粒组件的鉴定方面有大量发现,但动粒功能背后的物理相互作用仍不清楚。为了更好地理解动粒如何附着于微管以及这种附着是如何被调控的,我们试图描述动粒蛋白之间的相互作用,特别是关于微管结合Dam1复合体的相互作用。Dam1复合体在染色体-纺锤体附着中起关键作用,并且是极光激酶Ipl1p对这种附着进行磷酸化调控的关键靶点。为了鉴定涉及Dam1复合体的蛋白质-蛋白质相互作用,以及Dam1p磷酸化状态对这些物理相互作用的影响,我们对Dam1p进行了全基因组双杂交筛选和一系列生化结合测定。对一个包含6000个酵母开放阅读框的文库进行双杂交筛选,鉴定出9种动粒蛋白作为与Dam1p相互作用的伙伴。从涉及Dam1复合体所有9个亚基和32种动粒蛋白的113次体外结合反应中,我们在Dam1复合体内发现了至少9种相互作用以及Dam1复合体的19个潜在伙伴。引人注目的是,我们发现模拟Ipl1p位点磷酸化的突变会削弱Dam1p-Ndc80p和Dam1p-Spc34p的相互作用,这使我们能够构建一个磷酸化调控对动粒功能影响的模型。