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与酿酒酵母RAT2/NUP120基因突变相关的核孔复合体聚集及多聚腺苷酸(poly(A)+)RNA的核内积累

Nuclear pore complex clustering and nuclear accumulation of poly(A)+ RNA associated with mutation of the Saccharomyces cerevisiae RAT2/NUP120 gene.

作者信息

Heath C V, Copeland C S, Amberg D C, Del Priore V, Snyder M, Cole C N

机构信息

Department of Biochemistry, Dartmouth Medical School, Hanover, New Hampshire 03755, USA.

出版信息

J Cell Biol. 1995 Dec;131(6 Pt 2):1677-97. doi: 10.1083/jcb.131.6.1677.

Abstract

To identify genes involved in the export of messenger RNA from the nucleus to the cytoplasm, we used an in situ hybridization assay to screen temperature-sensitive strains of Saccharomyces cerevisiae. This identified those which accumulated poly(A)+ RNA in their nuclei when shifted to the non-permissive temperature of 37 degrees C. We describe here the properties of yeast strains carrying mutations in the RAT2 gene (RAT - ribonucleic acid trafficking) and the cloning of the RAT2 gene. Only a low percentage of cells carrying the rat2-1 allele showed nuclear accumulation of poly(A)+ RNA when cultured at 15 degrees or 23 degrees C, but within 4 h of a shift to the nonpermissive temperature of 37 degrees C, poly(A)+ RNA accumulated within the nuclei of approximately 80% of cells. No defect was seen in the nuclear import of a reporter protein bearing a nuclear localization signal. Nuclear pore complexes (NPCs) are distributed relatively evenly around the nuclear envelope in wild-type cells. In cells carrying either the rat2-1 or rat2-2 allele, NPCs were clustered together into one or a few regions of the nuclear envelope. This clustering was a constitutive property of mutant cells. NPCs remained clustered in crude nuclei isolated from mutant cells, indicating that these clusters are not able to redistribute around the nuclear envelope when nuclei are separated from cytoplasmic components. Electron microscopy revealed that these clusters were frequently found in a protuberance of the nuclear envelope and were often located close to the spindle pole body. The RAT2 gene encodes a 120-kD protein without similarity to other known proteins. It was essential for growth only at 37 degrees C, but the growth defect at high temperature could be suppressed by growth of mutant cells in the presence of high osmolarity media containing 1.0 M sorbitol or 0.9 M NaCl. The phenotypes seen in cells carrying a disruption of the RAT2 gene were very similar to those seen with the rat2-1 and rat2-2 alleles. Epitope tagging was used to show that Rat2p is located at the nuclear periphery and co-localizes with yeast NPC proteins recognized by the RL1 monoclonal antibody. The rat2-1 allele was synthetically lethal with both the rat3-1/nup133-1 and rat7-1/nup159-1 alleles. These results indicate that the product of this gene is a nucleoporin which we refer to as Rat2p/Nup120p.

摘要

为了鉴定参与信使核糖核酸从细胞核输出到细胞质过程的基因,我们利用原位杂交试验筛选酿酒酵母的温度敏感型菌株。这鉴定出了那些在转移到37℃的非允许温度时在细胞核中积累多聚腺苷酸(poly(A)+)RNA的菌株。我们在此描述携带RAT2基因(RAT - 核糖核酸运输)突变的酵母菌株的特性以及RAT2基因的克隆。当在15℃或23℃培养时,只有低比例携带rat2-1等位基因的细胞显示多聚腺苷酸(poly(A)+)RNA在细胞核中积累,但在转移到37℃的非允许温度后的4小时内,约80%的细胞的细胞核中积累了多聚腺苷酸(poly(A)+)RNA。在携带带有核核定位信号的报告蛋白的细胞核输入过程中未观察到缺陷。在野生型细胞中,核孔复合体(NPCs)相对均匀地分布在核膜周围。在携带rat2-1或rat2-2等位基因的细胞中,NPCs聚集在一起形成核膜的一个或几个区域。这种聚集是突变细胞的一个组成特性。NPCs在从突变细胞分离的粗制细胞核中仍然聚集,这表明当细胞核与细胞质成分分离时,这些聚集物不能在核膜周围重新分布。电子显微镜显示这些聚集物经常出现在核膜的一个突起中,并且经常位于靠近纺锤极体的位置。RAT2基因编码一种120-kD的蛋白质,与其他已知蛋白质没有相似性。它仅在37℃时对生长是必需的,但在含有1.0 M山梨醇或0.9 M氯化钠的高渗培养基中培养突变细胞可以抑制高温下的生长缺陷。在携带RAT2基因破坏的细胞中观察到的表型与在rat2-1和rat2-2等位基因中观察到的非常相似。表位标签用于显示Rat2p位于核周边并且与RL1单克隆抗体识别的酵母NPC蛋白共定位。rat2-1等位基因与rat3-1/nup133-1和rat7-1/nup159-1等位基因都是合成致死的。这些结果表明该基因的产物是一种核孔蛋白,我们将其称为Rat2p/Nup120p。

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本文引用的文献

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Trends Cell Biol. 1994 Oct;4(10):357-65. doi: 10.1016/0962-8924(94)90085-x.
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