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酿酒酵母中,与60S核糖体亚基前体相关的因子Arx1的核循环依赖于Rei1。

Nuclear recycling of the pre-60S ribosomal subunit-associated factor Arx1 depends on Rei1 in Saccharomyces cerevisiae.

作者信息

Hung Nai-Jung, Johnson Arlen W

机构信息

Section of Molecular Genetics and Microbiology and Institute for Cellular and Molecular Biology, 1 University Station, A5000, The University of Texas at Austin, Austin, Texas 78712-0162, USA.

出版信息

Mol Cell Biol. 2006 May;26(10):3718-27. doi: 10.1128/MCB.26.10.3718-3727.2006.

Abstract

Arx1 and Rei1 are found on late pre-60S ribosomal particles containing the export adaptor Nmd3. Arx1 is related to methionine aminopeptidases (MetAPs), and Rei1 is a C2H2 zinc finger protein whose function in ribosome biogenesis has not been previously characterized. Arx1 and Rei1 localized predominately to the nucleus and cytoplasm, respectively, but could be coimmunoprecipitated, suggesting that they are transiently in the same 60S complex. arx1delta mutants showed a modest accumulation of 60S subunits in the nucleus, suggesting that Arx1 enhances 60S export. Deletion of REI1 led to cold sensitivity and redistribution of Arx1 to the cytoplasm, where it remained bound to free 60S subunits. However, deletion of ARX1 or the fusion of enhanced GFP (eGFP) to Rpl25 suppressed the cold sensitivity of an rei1delta mutant. The presence of eGFP on Rpl25 or its neighboring protein Rpl35 reduced the binding of Arx1 to 60S subunits, suggesting that Arx1 binds to 60S subunits in the vicinity of the exit tunnel. Mutations in Arx1 that disrupted its binding to 60S also suppressed an rei1delta mutant and restored the normal nuclear localization of Arx1. These results indicate that the cold sensitivity of rei1delta cells is due to the persistence of Arx1 on 60S subunits in the cytoplasm. Furthermore, these results suggest that Rei1 is needed for release of Arx1 from nascent 60S subunits after export to the cytoplasm but not for the subsequent nuclear import of Arx1.

摘要

Arx1和Rei1存在于含有输出衔接蛋白Nmd3的晚期60S前核糖体颗粒上。Arx1与甲硫氨酸氨肽酶(MetAPs)相关,而Rei1是一种C2H2锌指蛋白,其在核糖体生物发生中的功能此前尚未得到表征。Arx1和Rei1分别主要定位于细胞核和细胞质,但可通过免疫共沉淀法检测到,这表明它们会短暂存在于同一个60S复合物中。arx1delta突变体在细胞核中显示出60S亚基的适度积累,这表明Arx1增强了60S的输出。REI1的缺失导致冷敏感性以及Arx1重新分布到细胞质中,在那里它仍然与游离的60S亚基结合。然而,ARX1的缺失或增强型绿色荧光蛋白(eGFP)与Rpl25的融合抑制了rei1delta突变体的冷敏感性。Rpl25或其相邻蛋白Rpl35上存在eGFP会降低Arx1与60S亚基的结合,这表明Arx1在出口通道附近与60S亚基结合。破坏Arx1与60S结合的突变也抑制了rei1delta突变体,并恢复了Arx1的正常核定位。这些结果表明,rei1delta细胞的冷敏感性是由于Arx1在细胞质中60S亚基上的持续存在。此外,这些结果表明,Rei1是Arx1在输出到细胞质后从新生60S亚基释放所必需的,但不是Arx1随后进行核输入所必需的。

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