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酿酒酵母60S核糖体生物合成GTP酶Nog1的体内功能特性分析

In vivo functional characterization of the Saccharomyces cerevisiae 60S biogenesis GTPase Nog1.

作者信息

Fuentes Jennifer L, Datta Kaustuv, Sullivan Susan M, Walker Angela, Maddock Janine R

机构信息

Department of Molecular, Cellular and Developmental Biology, University of Michigan, 830 North University Avenue, Ann Arbor, MI 48109, USA.

出版信息

Mol Genet Genomics. 2007 Jul;278(1):105-23. doi: 10.1007/s00438-007-0233-1. Epub 2007 Apr 19.

DOI:10.1007/s00438-007-0233-1
PMID:17443350
Abstract

The Saccharomyces cerevisiae Nog1 GTPase is critical for assembly of the large ribosomal subunit. Mutations in conserved residues in the GTP-binding pocket cause defects in cell growth and 60S ribosome assembly but mutant proteins retain their ability to associate with the pre-60S. Association of Nog1 with the pre-60S is independent of guanine nucleotide added to cell extracts. Thus, it appears that nucleotide occupancy does not substantially affect Nog1 association with pre-60S particles. Somewhat surprisingly, neither of the conserved threonines in the G2 motif of the GTPase domain is essential for Nog1 function. Neither the steady-state rRNA levels nor the protein composition (as determined by isobaric labeling and identification by mass spectrometry of peptides) of the pre-60S particles in the nog1P176V mutant are grossly perturbed, although levels of four proteins (Nog1, Nop2, Nop15, and Tif6) are modestly reduced in pre-60S particles isolated from the mutant. Deletion analysis revealed that the C-terminal 168 amino acids are not required for function; however, the N-terminal 126 amino acids are required. Optimal association with pre-60S particles requires sequences between amino acids 347-456. Several conserved charge-to-alanine substitutions outside the GTPase domain display modest growth phenotypes indicating that these residues are not critical for function.

摘要

酿酒酵母Nog1 GTP酶对于大核糖体亚基的组装至关重要。GTP结合口袋中保守残基的突变会导致细胞生长和60S核糖体组装缺陷,但突变蛋白仍保留其与前60S结合的能力。Nog1与前60S的结合不依赖于添加到细胞提取物中的鸟嘌呤核苷酸。因此,似乎核苷酸占据情况对Nog1与前60S的结合没有实质性影响。有点令人惊讶的是,GTP酶结构域G2基序中的两个保守苏氨酸对Nog1功能都不是必需的。nog1P176V突变体中前60S颗粒的稳态rRNA水平和蛋白质组成(通过等压标记和肽段质谱鉴定确定)均未受到严重干扰,尽管从突变体中分离的前60S颗粒中四种蛋白质(Nog1、Nop2、Nop15和Tif6)的水平略有降低。缺失分析表明,C末端的168个氨基酸对功能不是必需的;然而,N末端的126个氨基酸是必需的。与前60S颗粒的最佳结合需要氨基酸347 - 456之间的序列。GTP酶结构域之外的几个保守的电荷到丙氨酸的取代显示出适度的生长表型,表明这些残基对功能不是关键的。

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