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Pds1p对于酿酒酵母中后期的准确执行是必需的。

Pds1p is required for faithful execution of anaphase in the yeast, Saccharomyces cerevisiae.

作者信息

Yamamoto A, Guacci V, Koshland D

机构信息

Carnegie Institution of Washington, Department of Embryology, Baltimore, Maryland 21210, USA.

出版信息

J Cell Biol. 1996 Apr;133(1):85-97. doi: 10.1083/jcb.133.1.85.

Abstract

To identify mutations that cause defects in mitosis, a collection of mutants in Saccharomyces cerevisiae was screened by a rapid visual assay for abnormal chromosome segregation. From this screen we identified one mutation, pds1-1 that was independently identified in an alternative screen for mutants that exhibit inviability after transient exposure to nocodazole and precocious disassociation of sister chromatids (Guacci, V., A. Yamamoto, A. Strunnikov, J. Kingsbury, E. Hogan, P. Meluh, and D. Koshland. 1993. CSH Symp. Quant. Biol. 58:677-685; Yamamoto, T.J., G. Li, B. Schaar, I. Szilak, and D.W. Cleveland. 1992. Nature (Lond.). 359:536-539). At 23 degrees C pds1-1 mutants exhibit frequent cell death and a 300-fold increase in chromosome loss compared to wild type. At 37 degrees C pds1-1 cells fail to elongate their spindles during anaphase. This spindle defect of pds1 mutants results from a temperature-sensitive step that occurs around the G1/S boundary about the time of spindle assembly. In the absence of spindle elongation pds1 mutants undergo cytokinesis, leading to the missegregation of both chromosomes and spindle pole bodies. After abnormal cell division pds1-1 mutants also initiate new rounds of DNA replication, spindle pole body duplication, and bud formation. Thus, in the pds1-1 mutant at 37 degrees C, cell cycle progression is uncoupled from the completion of anaphase. A pds1 deletion allele has similar phenotypes to the original allele. Taken together these results suggest that Pds1 protein plays an important role in chromosome segregation at 23 degrees C and an essential role for this process at 37 degrees C. The PDS1 gene encodes a novel 42-kD nuclear protein that has both basic and acidic domains. The level of PDS1 mRNA varies with the cell cycle with maximal accumulation around the G1/S boundary. The stability of Pds1 protein also appears to change during the cell cycle as overproduced Pds1p is stable in S and M but degraded in early G1. Therefore, expression of Pds1p is regulated apparently both transcriptionally and postranslationally during the cell cycle. The phenotypes of pds1 mutants and expression pattern of Pds1p are discussed in the context of other spindle-defective mutants and the knowledge that Pds1 protein is an inhibitor of anaphase (Yamamoto, T.J., G. Li, B. Schaar, I. Szilak, and D.W. Cleveland. 1992. Nature (Lond.). 359:536-539).

摘要

为了鉴定导致有丝分裂缺陷的突变,通过一种用于检测异常染色体分离的快速视觉检测法,对酿酒酵母中的一组突变体进行了筛选。通过该筛选,我们鉴定出一个突变体pds1-1,它在另一个筛选中被独立鉴定出来,该筛选针对的是短暂暴露于诺考达唑后表现出不可存活性以及姐妹染色单体过早解离的突变体(瓜奇,V.,A. 山本,A. 斯特鲁尼科夫,J. 金斯伯里,E. 霍根,P. 梅卢,和D. 科什兰德。1993年。《定量生物学冷泉港研讨会》58:677 - 685;山本,T.J.,G. 李,B. 沙尔,I. 齐拉克,和D.W. 克利夫兰。1992年。《自然》(伦敦)。359:536 - 539)。在23摄氏度时,与野生型相比,pds1-1突变体表现出频繁的细胞死亡以及染色体丢失增加300倍。在37摄氏度时,pds1-1细胞在后期无法延长其纺锤体。pds1突变体的这种纺锤体缺陷源于大约在纺锤体组装时G1/S边界附近发生的一个温度敏感步骤。在没有纺锤体延长的情况下,pds1突变体进行胞质分裂,导致染色体和纺锤极体的错误分离。异常细胞分裂后,pds1-1突变体还会启动新一轮的DNA复制、纺锤极体复制和芽形成。因此,在37摄氏度的pds1-1突变体中,细胞周期进程与后期的完成脱钩。一个pds1缺失等位基因具有与原始等位基因相似的表型。综合这些结果表明,Pds1蛋白在23摄氏度时对染色体分离起重要作用,而在37摄氏度时对该过程起关键作用。PDS1基因编码一种新型的42-kD核蛋白,该蛋白具有碱性和酸性结构域。PDS1 mRNA的水平随细胞周期而变化,在G1/S边界附近积累达到最大值。Pds1蛋白的稳定性在细胞周期中似乎也会发生变化,因为过量产生的Pds1p在S期和M期稳定,但在G1早期会降解。因此,Pds1p的表达在细胞周期中显然受到转录和翻译后调控。在其他纺锤体缺陷突变体的背景下,以及基于Pds1蛋白是后期抑制剂这一知识,讨论了pds1突变体的表型和Pds1p的表达模式(山本,T.J.,G. 李,B. 沙尔,I. 齐拉克,和D.W. 克利夫兰。1992年。《自然》(伦敦)。359:536 - 539)。

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