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酵母线粒体依赖 tRNA 的氨酰基转移酶连接亚基 Gtf1p 的特性。

Characterization of Gtf1p, the connector subunit of yeast mitochondrial tRNA-dependent amidotransferase.

机构信息

Department of Microbiology, University of São Paulo, 05508-900 São Paulo, Brazil.

出版信息

J Biol Chem. 2011 Sep 23;286(38):32937-47. doi: 10.1074/jbc.M111.265371. Epub 2011 Jul 28.

Abstract

The bacterial GatCAB operon for tRNA-dependent amidotransferase (AdT) catalyzes the transamidation of mischarged glutamyl-tRNA(Gln) to glutaminyl-tRNA(Gln). Here we describe the phenotype of temperature-sensitive (ts) mutants of GTF1, a gene proposed to code for subunit F of mitochondrial AdT in Saccharomyces cerevisiae. The ts gtf1 mutants accumulate an electrophoretic variant of the mitochondrially encoded Cox2p subunit of cytochrome oxidase and an unstable form of the Atp8p subunit of the F(1)-F(0) ATP synthase that is degraded, thereby preventing assembly of the F(0) sector. Allotopic expression of recoded ATP8 and COX2 did not significantly improve growth of gtf1 mutants on respiratory substrates. However, ts gft1 mutants are partially rescued by overexpression of PET112 and HER2 that code for the yeast homologues of the catalytic subunits of bacterial AdT. Additionally, B66, a her2 point mutant has a phenotype similar to that of gtf1 mutants. These results provide genetic support for the essentiality, in vivo, of the GatF subunit of the heterotrimeric AdT that catalyzes formation of glutaminyl-tRNA(Gln) (Frechin, M., Senger, B., Brayé, M., Kern, D., Martin, R. P., and Becker, H. D. (2009) Genes Dev. 23, 1119-1130).

摘要

细菌 GatCAB 操纵子用于 tRNA 依赖性氨酰转移酶 (AdT) 催化错误负载的谷氨酰-tRNA(Gln) 向谷氨酰基-tRNA(Gln) 的转酰胺作用。在这里,我们描述了 GTF1 的温度敏感 (ts) 突变体的表型,GTF1 基因被提议编码酿酒酵母线粒体 AdT 的亚基 F。ts gtf1 突变体积累了细胞色素氧化酶的线粒体编码 Cox2p 亚基的电泳变体和不稳定形式的 F(1)-F(0)ATP 合酶的 Atp8p 亚基,该亚基被降解,从而阻止 F(0) 部分的组装。重编码的 ATP8 和 COX2 的异位表达并没有显著改善 gtf1 突变体在呼吸底物上的生长。然而,PET112 和 HER2 的过表达部分挽救了 gft1 突变体,它们编码细菌 AdT 的催化亚基的酵母同源物。此外,her2 点突变体 B66 的表型类似于 gtf1 突变体。这些结果为催化形成谷氨酰基-tRNA(Gln)的异三聚体 AdT 的 GatF 亚基在体内的必要性提供了遗传支持 (Frechin, M., Senger, B., Brayé, M., Kern, D., Martin, R. P., and Becker, H. D. (2009) Genes Dev. 23, 1119-1130)。

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