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从ELT细胞中分离核仁:一种能保持形态完整性和高转录活性的快速新方法。

Isolation of nucleoli from ELT cells: a quick new method that preserves morphological integrity and high transcriptional activity.

作者信息

Vandelaer M, Thiry M, Goessens G

机构信息

Laboratory of Cell and Tissue Biology, Faculty of Sciences, University of Liège, Belgium.

出版信息

Exp Cell Res. 1996 Oct 10;228(1):125-31. doi: 10.1006/excr.1996.0307.

Abstract

We have developed a quick new method for isolating nucleoli which, unlike the methods in current use, preserves the nucleolar ultrastructure. Until now, the isolation process has generally been assumed to empty one of the three major compartments of the nucleolus, the fibrillar center, of its content. We have used the AgNOR staining and in vitro transcription assay to test the degree of structural and functional preservation of the isolated nucleoli. Our results demonstrate the value of our procedure as a reliable tool for biochemical and ultrastructural studies on the nucleolus. Moreover, these proprieties prompt us to investigate the rRNA synthesis, using a nonisotopic approach, within morphologically intact isolated nucleoli. Thus, we show that newly synthesized rRNA transcripts are located not only in the dense fibrillar component, but also indubitably in the fibrillar center.

摘要

我们开发了一种快速的新方法来分离核仁,与目前使用的方法不同,该方法能保留核仁的超微结构。到目前为止,一般认为分离过程会使核仁三个主要区域之一的纤维中心的内容物排空。我们使用了银染核仁组织区染色和体外转录试验来测试分离核仁的结构和功能保存程度。我们的结果证明了我们的方法作为一种用于核仁生化和超微结构研究的可靠工具的价值。此外,这些特性促使我们使用非同位素方法在形态完整的分离核仁内研究核糖体RNA合成。因此,我们表明新合成的核糖体RNA转录本不仅位于致密纤维组分中,而且无疑也位于纤维中心。

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