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鉴定tRNA结合蛋白Arc1p为酿酒酵母体内生物素化的新靶点。

Identification of the tRNA-binding protein Arc1p as a novel target of in vivo biotinylation in Saccharomyces cerevisiae.

作者信息

Kim Hyun Soo, Hoja Ursula, Stolz Juergen, Sauer Guido, Schweizer Eckhart

机构信息

Lehrstuhl für Biochemie der Universität Erlangen-Nürnberg, Erlangen D-91058, Germany.

出版信息

J Biol Chem. 2004 Oct 8;279(41):42445-52. doi: 10.1074/jbc.M407137200. Epub 2004 Jul 22.

DOI:10.1074/jbc.M407137200
PMID:15272000
Abstract

Biotin is an essential cofactor of cell metabolism serving as a protein-bound coenzyme in ATP-dependent carboxylation, in transcarboxylation, and certain decarboxylation reactions. The involvement of biotinylated proteins in other cellular functions has been suggested occasionally, but available data on this are limited. In the present study, a Saccharomyces cerevisiae protein was identified that reacts with streptavidin on Western blots and is not identical to one of the known biotinylated yeast proteins. After affinity purification on monomeric avidin, the biotinylated protein was identified as Arc1p. Using 14C-labeled biotin, the cofactor was shown to be incorporated into Arc1p by covalent and alkali-stable linkage. Similar to the known carboxylases, Arc1p biotinylation is mediated by the yeast biotin:protein ligase, Bpl1p. Mutational studies revealed that biotinylation occurs at lysine 86 within the N-terminal domain of Arc1p. In contrast to the known carboxylases, however, in vitro biotinylation of Arc1p is incomplete and increases with BPL1 overexpression. In accordance to this fact, Arc1p lacks the canonical consensus sequence of known biotin binding domains, and the bacterial biotin:protein ligase, BirA, is unable to use Arc1p as a substrate. Arc1p was shown previously to organize the association of MetRS and GluRS tRNA synthetases with their cognate tRNAs thereby increasing the substrate affinity and catalytic efficiency of these enzymes. Remarkably, not only biotinylated but also the biotin-free Arc1p obtained by replacement of lysine 86 with arginine were capable of restoring Arc1p function in both arc1Delta and arc1Deltalos1Delta mutants, indicating that biotinylation of Arc1p is not essential for activity.

摘要

生物素是细胞代谢的一种必需辅助因子,在ATP依赖性羧化反应、转羧化反应和某些脱羧反应中作为与蛋白质结合的辅酶。生物素化蛋白偶尔也被认为参与其他细胞功能,但关于这方面的现有数据有限。在本研究中,鉴定出一种酿酒酵母蛋白,它在蛋白质免疫印迹法中与抗生物素蛋白链菌素发生反应,且与已知的生物素化酵母蛋白之一不同。在单体抗生物素蛋白上进行亲和纯化后,该生物素化蛋白被鉴定为Arc1p。使用14C标记的生物素,显示该辅助因子通过共价且对碱稳定的连接方式掺入Arc1p中。与已知的羧化酶类似,Arc1p的生物素化由酵母生物素:蛋白质连接酶Bpl1p介导。突变研究表明,生物素化发生在Arc1p N端结构域内的赖氨酸86处。然而,与已知的羧化酶不同,Arc1p的体外生物素化不完全,且随着BPL1的过表达而增加。基于这一事实,Arc1p缺乏已知生物素结合结构域的典型共有序列,并且细菌生物素:蛋白质连接酶BirA不能将Arc1p用作底物。先前已表明Arc1p可组织甲硫氨酰-tRNA合成酶和谷氨酰胺-tRNA合成酶与其相应tRNA的结合,从而提高这些酶的底物亲和力和催化效率。值得注意的是,不仅生物素化的Arc1p,而且通过将赖氨酸86替换为精氨酸获得的无生物素Arc1p都能够在arc1Delta和arc1Deltalos1Delta突变体中恢复Arc1p的功能,这表明Arc1p的生物素化对其活性并非必需。

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