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首页> 外文期刊>The Journal of biological chemistry >Identification of Pep4p as the Protease Responsible for Formation of the SAGA-related SLIK Protein Complex
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Identification of Pep4p as the Protease Responsible for Formation of the SAGA-related SLIK Protein Complex

机译:鉴定Pep4P作为负责形成佐贺相关的Slik蛋白复合物的蛋白酶

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The Saccharomyces cerevisiae Spt-Ada-Gcn5 acetyltransferase (SAGA) protein complex is a coactivator for transcription by RNA polymerase II and has various activities, including acetylation and deubuiqitination of histones and recruitment of TATA-binding protein to promoters. The Spt7p subunit is subject to proteolytic cleavage at its C terminus resulting in removal of the Spt8p-binding domain and generation of the SAGA-related SALSA/SAGA-like (SLIK) protein complex. Here, we report identification of the protease responsible for this cleavage. Screening of a protease knock-out collection revealed PEP4 to be required for cleavage of Spt7p within SAGA in vitro. Endogenous formation of truncated Spt7p was abolished in cells lacking PEP4. Purified Pep4p but not catalytic dead mutant Pep4p or unrelated Prc1p protease specifically cleaved Spt7p within SAGA into SLIK-related Spt7p. Interestingly, SAGA lacking Spt8p was more sensitive to Pep4p-mediated truncation of Spt7p, suggesting that Spt8p counteracted its own release from SAGA. Strains mimicking constitutive SLIK formation showed increased resistance to rapamycin treatment, suggesting a role for SLIK in regulating cellular responses to nutrient stress.
机译:酿酒酵母SPT-ADA-GCN5乙酰转移酶(SAGA)蛋白质复合物是用于RNA聚合酶II的转录的共觉器,并且具有各种活性,包括组蛋白的乙酰化和DeubuiQitination,并对TATA结合蛋白募集到启动子。 SPT7P亚基在其C末端受蛋白水解裂解,导致去除SPT8P结合结构域并产生佐贺相关的SAGA / SAGA样(SLIK)蛋白质复合物。在这里,我们报告鉴定负责这种裂解的蛋白酶。筛选蛋白酶敲除收集的筛选揭示了Pep4,以在体外佐贺中切割SPT7P。在缺乏Pep4的细胞中消除了截短的SPT7P的内源性形成。纯化的Pep4P但不催化死突变体Pep4P或不相关的PRC1P蛋白酶在SAGA内特别切割SPT7p进入Slik相关的SPT7P。有趣的是,缺乏SPT8P的SAGA对PEP4P介导的SPT7P截断更敏感,这表明SPT8P抵消了SAGA的自身释放。模仿组成型Slik形成的菌株显示出对雷帕霉素治疗的抗性增加,表明Slik在调节对营养应激的细胞反应中的角色作用。

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