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酵母tra1的磷脂酰肌醇-3-激酶结构域的结构/功能分析

Structure/function analysis of the phosphatidylinositol-3-kinase domain of yeast tra1.

作者信息

Mutiu A Irina, Hoke Stephen M T, Genereaux Julie, Hannam Carol, MacKenzie Katherine, Jobin-Robitaille Olivier, Guzzo Julie, Côté Jacques, Andrews Brenda, Haniford David B, Brandl Christopher J

机构信息

Department of Biochemistry, Schulich School of Medicine and Dentistry, University of Western Ontario, London, Ontario N6A5C1, Canada.

出版信息

Genetics. 2007 Sep;177(1):151-66. doi: 10.1534/genetics.107.074476. Epub 2007 Jul 29.

Abstract

Tra1 is an essential component of the Saccharomyces cerevisiae SAGA and NuA4 complexes. Using targeted mutagenesis, we identified residues within its C-terminal phosphatidylinositol-3-kinase (PI3K) domain that are required for function. The phenotypes of tra1-P3408A, S3463A, and SRR3413-3415AAA included temperature sensitivity and reduced growth in media containing 6% ethanol or calcofluor white or depleted of phosphate. These alleles resulted in a twofold or greater change in expression of approximately 7% of yeast genes in rich media and reduced activation of PHO5 and ADH2 promoters. Tra1-SRR3413 associated with components of both the NuA4 and SAGA complexes and with the Gal4 transcriptional activation domain similar to wild-type protein. Tra1-SRR3413 was recruited to the PHO5 promoter in vivo but gave rise to decreased relative amounts of acetylated histone H3 and histone H4 at SAGA and NuA4 regulated promoters. Distinct from other components of these complexes, tra1-SRR3413 resulted in generation-dependent telomere shortening and synthetic slow growth in combination with deletions of a number of genes with roles in membrane-related processes. While the tra1 alleles have some phenotypic similarities with deletions of SAGA and NuA4 components, their distinct nature may arise from the simultaneous alteration of SAGA and NuA4 functions.

摘要

Tra1是酿酒酵母SAGA和NuA4复合物的一个重要组成部分。通过定向诱变,我们确定了其C端磷脂酰肌醇-3-激酶(PI3K)结构域内功能所需的残基。tra1-P3408A、S3463A和SRR3413-3415AAA的表型包括温度敏感性以及在含有6%乙醇、荧光增白剂或缺乏磷酸盐的培养基中生长减缓。这些等位基因导致丰富培养基中约7%的酵母基因表达发生两倍或更大的变化,并降低了PHO5和ADH2启动子的激活。Tra1-SRR3413与NuA4和SAGA复合物的成分以及与野生型蛋白相似的Gal4转录激活结构域相关。Tra1-SRR3413在体内被募集到PHO5启动子,但在SAGA和NuA4调控的启动子处导致乙酰化组蛋白H3和组蛋白H4的相对量减少。与这些复合物的其他成分不同,tra1-SRR3413导致依赖世代的端粒缩短,并与许多在膜相关过程中起作用的基因缺失相结合产生合成性生长缓慢。虽然tra1等位基因与SAGA和NuA4成分缺失有一些表型相似性,但其独特性质可能源于SAGA和NuA4功能的同时改变。

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