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在染色质铺展中对高度转录的rRNA基因新生转录本进行超微结构原位杂交。

Ultrastructural in situ hybridization to nascent transcripts of highly transcribed rRNA genes in chromatin spreads.

作者信息

O'Reilly M M, French S L, Sikes M L, Miller O L

机构信息

Department of Biology, University of Virginia, Charlottesville 22903.

出版信息

Chromosoma. 1994 Apr;103(2):122-8. doi: 10.1007/BF00352321.

Abstract

The amplified rRNA genes of amphibian oocytes were used as a model system for the development of an in situ hybridization technique to label nascent transcripts in dispersed chromatin. A biotinylated complementary RNA probe was hybridized to nascent transcripts from dispersed nucleoli, and detected by a two step antibody technique utilizing colloidal gold as an electron dense marker. A specific sequence on the rRNA nascent transcript was labeled in a pattern consistent with its location; however, gene morphology was difficult to analyze following in situ hybridization owing to low sample contrast. Proteins associated with the transcripts were apparently lost during the procedure, leading to decreased electron density of the transcripts. The technique was systematically modified in an attempt to identify conditions that preserved gene morphology adequately for ultrastructural analysis, while simultaneously maintaining sufficient levels of specific labeling.

摘要

两栖动物卵母细胞的扩增核糖体RNA基因被用作一个模型系统,用于开发一种原位杂交技术,以标记分散染色质中的新生转录本。将生物素化的互补RNA探针与分散核仁中的新生转录本杂交,并通过利用胶体金作为电子致密标记的两步抗体技术进行检测。核糖体RNA新生转录本上的特定序列以与其位置一致的模式被标记;然而,由于样品对比度低,原位杂交后基因形态难以分析。与转录本相关的蛋白质在该过程中明显丢失,导致转录本的电子密度降低。该技术经过系统改进,试图确定能够充分保留基因形态以进行超微结构分析的条件,同时保持足够水平的特异性标记。

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