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Sm蛋白和U2B”蛋白在休眠和增殖的洋葱细胞中重新分布到不同的核区域。

Sm and U2B" proteins redistribute to different nuclear domains in dormant and proliferating onion cells.

作者信息

Cui Ping, Moreno Díaz de la Espina Susana

机构信息

Nuclear Matrix Laboratory, Department of Plant Biology, Centro de Investigaciones Biológicas, CSIC, Velázquez 144, 28006, Madrid, Spain.

出版信息

Planta. 2003 May;217(1):21-31. doi: 10.1007/s00425-002-0966-3. Epub 2003 Jan 25.

DOI:10.1007/s00425-002-0966-3
PMID:12721845
Abstract

Monoclonal antibodies against the spliceosomal proteins Sm and U2B", and against p105, a protein component of interchromatin granules, were used to investigate the nuclear distribution of the splicing factors in Allium cepa L. meristematic cells. Confocal microscopy showed that in steady-state proliferating cells, the spliceosomal components were distributed into two nuclear domains: (i) a diffuse nucleoplasmic network similar to that formed by interchromatin granules and (ii) numerous Cajal bodies. These domains were the counterpart of the perichromatin fibrils and granules, interchromatin granules and Cajal bodies observed by electron microscopy after EDTA and bismuth oxynitrate stainings. Dormant cells showed a nuclear distribution of the proteins in small Cajal bodies and numerous micro-speckles, correlated with the distribution of ribonucleoproteins (RNPs) observed by electron microscopy. The spliceosomal proteins relocated to the diffuse nucleoplasmic network and Cajal bodies when the cells were released from dormancy by water soaking and they re-started their proliferative activity. Inhibition of RNA synthesis by 5,6-dichloro-1-beta- d-ribofuranosylbenzimidazole (DRB) treatment in proliferating cells demonstrated that the micro-speckles were not the morphological expression of a transcription block. Fractionation and confocal microscopy studies showed a differential association of the splicing factors with the nuclear matrix depending not only on the protein, but also on nuclear activity. Our results suggest a reversible relocation of the spliceosomal proteins between different sub-nuclear domains in physiological conditions. We report here an unusual nuclear domain in dormant nuclei, the micro-speckles, corresponding to storage sites for RNPs, which were rapidly mobilised after water imbibition.

摘要

针对剪接体蛋白Sm和U2B"以及染色质间颗粒的一种蛋白成分p105的单克隆抗体,被用于研究葱属植物分生组织细胞中剪接因子的核分布。共聚焦显微镜显示,在稳态增殖细胞中,剪接体成分分布于两个核区域:(i) 一个类似于由染色质间颗粒形成的弥散核质网络,以及 (ii) 众多的卡哈尔体。这些区域与经乙二胺四乙酸(EDTA)和硝酸氧铋染色后电子显微镜观察到的染色质周纤维和颗粒、染色质间颗粒及卡哈尔体相对应。休眠细胞中这些蛋白在小卡哈尔体和众多微斑点中呈现核分布,这与电子显微镜观察到的核糖核蛋白(RNP)分布相关。当通过水浸使细胞从休眠中释放并重新开始增殖活动时,剪接体蛋白重新定位到弥散核质网络和卡哈尔体。在增殖细胞中用5,6 - 二氯 - 1 - β - D - 呋喃核糖基苯并咪唑(DRB)处理抑制RNA合成表明,微斑点并非转录阻滞的形态学表现。分级分离和共聚焦显微镜研究表明,剪接因子与核基质的关联存在差异,这不仅取决于蛋白,还取决于核活性。我们的结果表明,在生理条件下剪接体蛋白可在不同的亚核区域之间进行可逆性重新定位。我们在此报告了休眠细胞核中一个不寻常的核区域,即微斑点,它对应于RNP的储存位点,在吸水后会迅速被调动起来。

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本文引用的文献

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