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本文引用的文献

1
Cdc14-regulated midzone assembly controls anaphase B.Cdc14调控的中间区组装控制后期B。
J Cell Biol. 2007 Jun 18;177(6):981-93. doi: 10.1083/jcb.200702145. Epub 2007 Jun 11.
2
Plus end-specific depolymerase activity of Kip3, a kinesin-8 protein, explains its role in positioning the yeast mitotic spindle.驱动蛋白8家族蛋白Kip3的正端特异性解聚酶活性,解释了其在酵母有丝分裂纺锤体定位中的作用。
Nat Cell Biol. 2006 Sep;8(9):913-23. doi: 10.1038/ncb1457. Epub 2006 Aug 13.
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Gene function prediction from congruent synthetic lethal interactions in yeast.基于酵母中一致的合成致死相互作用进行基因功能预测。
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4
Asymmetric recruitment of dynein to spindle poles and microtubules promotes proper spindle orientation in yeast.动力蛋白向纺锤体极和微管的不对称募集促进了酵母中纺锤体的正确定向。
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The regulation of microtubule dynamics in Saccharomyces cerevisiae by three interacting plus-end tracking proteins.三种相互作用的正端追踪蛋白对酿酒酵母微管动力学的调控
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Arp10p is a pointed-end-associated component of yeast dynactin.Arp10p是酵母动力蛋白激活蛋白的一个指向末端相关成分。
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A genome-wide screen for Saccharomyces cerevisiae nonessential genes involved in mannosyl phosphate transfer to mannoprotein-linked oligosaccharides.一项全基因组筛选,寻找参与磷酸甘露糖转移至甘露糖蛋白连接寡糖过程的酿酒酵母非必需基因。
Fungal Genet Biol. 2005 Sep;42(9):773-90. doi: 10.1016/j.fgb.2005.05.002.
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NudEL targets dynein to microtubule ends through LIS1.NudEL通过LIS1将动力蛋白靶向微管末端。
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9
Systematic interpretation of genetic interactions using protein networks.利用蛋白质网络对基因相互作用进行系统解读。
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Spindle microtubules in flux.处于动态变化中的纺锤体微管。
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酿酒酵母中与p24同源的蛋白对于维持p150Glued与动力蛋白激活蛋白复合体的结合至关重要。

The Saccharomyces cerevisiae homolog of p24 is essential for maintaining the association of p150Glued with the dynactin complex.

作者信息

Amaro I Alexandra, Costanzo Michael, Boone Charles, Huffaker Tim C

机构信息

Department of Molecular Biology and Genetics, Cornell University, Ithaca, NY 14853, USA.

出版信息

Genetics. 2008 Feb;178(2):703-9. doi: 10.1534/genetics.107.079103. Epub 2008 Feb 1.

DOI:10.1534/genetics.107.079103
PMID:18245366
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2248349/
Abstract

Stu1 is the Saccharomyces cerevisiae member of the CLASP family of microtubule plus-end tracking proteins and is essential for spindle formation. A genomewide screen for gene deletions that are lethal in combination with the temperature-sensitive stu1-5 allele identified ldb18Delta. ldb18Delta cells exhibit defects in spindle orientation similar to those caused by a block in the dynein pathway. Consistent with this observation, ldb18Delta is synthetic lethal with mutations affecting the Kar9 spindle orientation pathway, but not with those affecting the dynein pathway. We show that Ldb18 is a component of dynactin, a complex required for dynein activity in yeast and mammalian cells. Ldb18 shares modest sequence and structural homology with the mammalian dynactin component p24. It interacts with dynactin proteins in two-hybrid and co-immunoprecipitation assays, and comigrates with them as a 20 S complex during sucrose gradient sedimentation. In ldb18Delta cells, the interaction between Nip100 (p150(Glued)) and Jnm1 (dynamitin) is disrupted, while the interaction between Jnm1 and Arp1 is not affected. These results indicate that p24 is required for attachment of the p150(Glued) arm to dynamitin and the remainder of the dynactin complex. The genetic interaction of ldb18Delta with stu1-5 also supports the notion that dynein/dynactin helps to generate a spindle pole separating force.

摘要

Stu1是微管正端追踪蛋白CLASP家族的酿酒酵母成员,对纺锤体形成至关重要。一项全基因组筛选,寻找与温度敏感型stu1-5等位基因组合时致死的基因缺失,鉴定出了ldb18Δ。ldb18Δ细胞在纺锤体定向方面表现出缺陷,类似于动力蛋白途径受阻所导致的缺陷。与这一观察结果一致,ldb18Δ与影响Kar9纺锤体定向途径的突变具有合成致死性,但与影响动力蛋白途径的突变没有合成致死性。我们发现Ldb18是动力蛋白激活复合物的一个组分,该复合物在酵母和哺乳动物细胞中对于动力蛋白活性是必需的。Ldb18与哺乳动物动力蛋白激活复合物组分p24有适度的序列和结构同源性。它在双杂交和共免疫沉淀试验中与动力蛋白激活复合物蛋白相互作用,并且在蔗糖梯度沉降过程中与它们一起以20 S复合物形式迁移。在ldb18Δ细胞中,Nip100(p150(Glued))和Jnm1(动力蛋白抑制因子)之间的相互作用被破坏,而Jnm1和Arp1之间的相互作用不受影响。这些结果表明,p24对于p150(Glued)臂与动力蛋白抑制因子以及动力蛋白激活复合物其余部分的附着是必需的。ldb18Δ与stu1-5的遗传相互作用也支持动力蛋白/动力蛋白激活复合物有助于产生纺锤体极分离力这一观点。