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Physiological importance and identification of novel targets for the N-terminal acetyltransferase NatB.N-末端乙酰转移酶NatB的生理重要性及新靶点的鉴定
Eukaryot Cell. 2006 Feb;5(2):368-78. doi: 10.1128/EC.5.2.368-378.2006.
2
The stress-induced Tfs1p requires NatB-mediated acetylation to inhibit carboxypeptidase Y and to regulate the protein kinase A pathway.应激诱导的Tfs1p需要NatB介导的乙酰化作用来抑制羧肽酶Y并调节蛋白激酶A途径。
J Biol Chem. 2004 Sep 10;279(37):38532-43. doi: 10.1074/jbc.M402939200. Epub 2004 Jun 30.
3
Nat3p and Mdm20p are required for function of yeast NatB Nalpha-terminal acetyltransferase and of actin and tropomyosin.酵母NatB Nα-末端乙酰转移酶以及肌动蛋白和原肌球蛋白的功能需要Nat3p和Mdm20p。
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Mdm20 protein functions with Nat3 protein to acetylate Tpm1 protein and regulate tropomyosin-actin interactions in budding yeast.Mdm20蛋白与Nat3蛋白共同发挥作用,使Tpm1蛋白乙酰化,并调节出芽酵母中的原肌球蛋白-肌动蛋白相互作用。
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Growth phase diets diminish histone acetyltransferase Gcn5 function and shorten lifespan of Drosophila males.生长期饮食会削弱组蛋白乙酰转移酶Gcn5的功能并缩短雄性果蝇的寿命。
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本文引用的文献

1
Dependence of ORC silencing function on NatA-mediated Nalpha acetylation in Saccharomyces cerevisiae.酿酒酵母中ORC沉默功能对NatA介导的Nα乙酰化的依赖性。
Mol Cell Biol. 2004 Dec;24(23):10300-12. doi: 10.1128/MCB.24.23.10300-10312.2004.
2
Importance of the Sir3 N terminus and its acetylation for yeast transcriptional silencing.Sir3蛋白N端及其乙酰化对酵母转录沉默的重要性。
Genetics. 2004 Sep;168(1):547-51. doi: 10.1534/genetics.104.028803.
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X-ray survival characteristics and genetic analysis for nine Saccharomyces deletion mutants that show altered radiation sensitivity.九个显示辐射敏感性改变的酿酒酵母缺失突变体的X射线存活特征及遗传分析。
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4
The stress-induced Tfs1p requires NatB-mediated acetylation to inhibit carboxypeptidase Y and to regulate the protein kinase A pathway.应激诱导的Tfs1p需要NatB介导的乙酰化作用来抑制羧肽酶Y并调节蛋白激酶A途径。
J Biol Chem. 2004 Sep 10;279(37):38532-43. doi: 10.1074/jbc.M402939200. Epub 2004 Jun 30.
5
Golgi targeting of ARF-like GTPase Arl3p requires its Nalpha-acetylation and the integral membrane protein Sys1p.Golgi靶向的ARF样GTP酶Arl3p需要其Nα-乙酰化和整合膜蛋白Sys1p。
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6
Targeting of the Arf-like GTPase Arl3p to the Golgi requires N-terminal acetylation and the membrane protein Sys1p.将类Arf GTP酶Arl3p靶向至高尔基体需要N端乙酰化作用和膜蛋白Sys1p。
Nat Cell Biol. 2004 May;6(5):405-13. doi: 10.1038/ncb1120. Epub 2004 Apr 11.
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A Snf2 family ATPase complex required for recruitment of the histone H2A variant Htz1.一种募集组蛋白H2A变体Htz1所需的Snf2家族ATP酶复合物。
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Global analysis of protein localization in budding yeast.芽殖酵母中蛋白质定位的全局分析。
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N-末端乙酰转移酶NatB的生理重要性及新靶点的鉴定

Physiological importance and identification of novel targets for the N-terminal acetyltransferase NatB.

作者信息

Caesar Robert, Warringer Jonas, Blomberg Anders

机构信息

Department of Cell and Molecular Biology, Lundberg Laboratory, Göteborg University, Medicinaregatan 9c, 413 90 Göteborg, Sweden.

出版信息

Eukaryot Cell. 2006 Feb;5(2):368-78. doi: 10.1128/EC.5.2.368-378.2006.

DOI:10.1128/EC.5.2.368-378.2006
PMID:16467477
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1405896/
Abstract

The N-terminal acetyltransferase NatB in Saccharomyces cerevisiae consists of the catalytic subunit Nat3p and the associated subunit Mdm20p. We here extend our present knowledge about the physiological role of NatB by a combined proteomics and phenomics approach. We found that strains deleted for either NAT3 or MDM20 displayed different growth rates and morphologies in specific stress conditions, demonstrating that the two NatB subunits have partly individual functions. Earlier reported phenotypes of the nat3Delta strain have been associated with altered functionality of actin cables. However, we found that point mutants of tropomyosin that suppress the actin cable defect observed in nat3Delta only partially restores wild-type growth and morphology, indicating the existence of functionally important acetylations unrelated to actin cable function. Predicted NatB substrates were dramatically overrepresented in a distinct set of biological processes, mainly related to DNA processing and cell cycle progression. Three of these proteins, Cac2p, Pac10p, and Swc7p, were identified as true NatB substrates. To identify N-terminal acetylations potentially important for protein function, we performed a large-scale comparative phenotypic analysis including nat3Delta and strains deleted for the putative NatB substrates involved in cell cycle regulation and DNA processing. By this procedure we predicted functional importance of the N-terminal acetylation for 31 proteins.

摘要

酿酒酵母中的N端乙酰转移酶NatB由催化亚基Nat3p和相关亚基Mdm20p组成。我们在此通过蛋白质组学和表型组学相结合的方法扩展了我们目前对NatB生理作用的认识。我们发现,缺失NAT3或MDM20的菌株在特定应激条件下表现出不同的生长速率和形态,这表明NatB的两个亚基具有部分独立的功能。先前报道的nat3Delta菌株的表型与肌动蛋白电缆功能的改变有关。然而,我们发现,抑制nat3Delta中观察到的肌动蛋白电缆缺陷的原肌球蛋白点突变体仅部分恢复野生型生长和形态,这表明存在与肌动蛋白电缆功能无关的功能重要的乙酰化作用。预测的NatB底物在一组独特的生物学过程中显著富集,主要与DNA加工和细胞周期进程有关。其中三种蛋白质Cac2p、Pac10p和Swc7p被鉴定为真正的NatB底物。为了鉴定对蛋白质功能可能重要的N端乙酰化作用,我们进行了大规模的比较表型分析,包括nat3Delta以及缺失参与细胞周期调控和DNA加工的假定NatB底物的菌株。通过这个过程,我们预测了31种蛋白质N端乙酰化的功能重要性。